CA2380202A1 - Novel crude and crystalline forms of lercanidipine hydrochloride - Google Patents
Novel crude and crystalline forms of lercanidipine hydrochloride Download PDFInfo
- Publication number
- CA2380202A1 CA2380202A1 CA 2380202 CA2380202A CA2380202A1 CA 2380202 A1 CA2380202 A1 CA 2380202A1 CA 2380202 CA2380202 CA 2380202 CA 2380202 A CA2380202 A CA 2380202A CA 2380202 A1 CA2380202 A1 CA 2380202A1
- Authority
- CA
- Canada
- Prior art keywords
- lercanidipine hydrochloride
- crude
- lercanidipine
- solid
- solvent
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Abandoned
Links
- WMFYOYKPJLRMJI-UHFFFAOYSA-N Lercanidipine hydrochloride Chemical compound Cl.COC(=O)C1=C(C)NC(C)=C(C(=O)OC(C)(C)CN(C)CCC(C=2C=CC=CC=2)C=2C=CC=CC=2)C1C1=CC=CC([N+]([O-])=O)=C1 WMFYOYKPJLRMJI-UHFFFAOYSA-N 0.000 title claims abstract description 205
- 229960002162 lercanidipine hydrochloride Drugs 0.000 title claims abstract description 149
- 238000000034 method Methods 0.000 claims abstract description 128
- 239000008194 pharmaceutical composition Substances 0.000 claims abstract description 22
- XEKOWRVHYACXOJ-UHFFFAOYSA-N Ethyl acetate Chemical compound CCOC(C)=O XEKOWRVHYACXOJ-UHFFFAOYSA-N 0.000 claims description 82
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- LFQSCWFLJHTTHZ-UHFFFAOYSA-N Ethanol Chemical compound CCO LFQSCWFLJHTTHZ-UHFFFAOYSA-N 0.000 claims description 70
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- XLYOFNOQVPJJNP-UHFFFAOYSA-N water Substances O XLYOFNOQVPJJNP-UHFFFAOYSA-N 0.000 claims description 52
- 239000002904 solvent Substances 0.000 claims description 42
- 229960004294 lercanidipine Drugs 0.000 claims description 41
- 238000003756 stirring Methods 0.000 claims description 40
- ZDXUKAKRHYTAKV-UHFFFAOYSA-N lercanidipine Chemical compound COC(=O)C1=C(C)NC(C)=C(C(=O)OC(C)(C)CN(C)CCC(C=2C=CC=CC=2)C=2C=CC=CC=2)C1C1=CC=CC([N+]([O-])=O)=C1 ZDXUKAKRHYTAKV-UHFFFAOYSA-N 0.000 claims description 38
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Landscapes
- Hydrogenated Pyridines (AREA)
Abstract
The invention is directed to novel crude forms and crystalline forms of lercanidipine hydrochloride, and to processes for the preparation of these forms.
Pharmaceutical compositions comprising the novel crystalline forms also are contemplated.
Pharmaceutical compositions comprising the novel crystalline forms also are contemplated.
Description
Docket No.: 648510J959-CAO
NOVEL CRUDE AND CRYSTALLINE FORMS OF LERCANIDIPINE
HYDROCHLORIDE
FIELD OF THE INVENTION
The invention is directed to novel crude forms and crystalline forms of lercanidipine hydrochloride, and to processes for the preparation of these forms.
Pharmaceutical compositions comprising the novel crystalline forms also are contemplated.
BACKGROUND OF THE INVENTION
Lercanidipine (methyl l,l;N-trimethyl-N-(3,3-diphenylpropyl)-2-aminoethyl 1,4-dihydro-2,6-dimethyl-4-(3-nitrophenyl)pyridine-3,5-dicarboxylate) is a highly lipophilic dihydropyridine calcium antagonist with long duration of action and high vascular selectivity.
Its mechanism of antihypertensive activity is attributed to a direct relaxant effect on vascular smooth muscle; which lowers total peripheral resistance. The recommended starting dose of lercanidipine as monotherapy is 10 mg daily by oral route, with a drug titration as necessary to 20 mg daily. Lercanidipine is rapidly absorbed following oral administration with peak plasma levels occurring 2-3 ;hours following dosing. Elimination is essentially via the hepatic route.
By virtue of its high lipophilicity and high membrane coefficient, lercanidipine combines a short;plasma half life with a long duration of action. In fact, the preferential distribution of the drug into membranes of smooth muscle cells results in membrane-controlled pharmacokinetics which is characterized by a prolonged pharmacological effect.
In comparison -v to other calcium antagonists, lercanidipine is characterized by gradual onset and long-lasting duration of action despite decreasing plasma levels. In vitro studies show that isolated rat aorta response to high K+' may be attenuated by lercanidipine, even after the drug has been removed from the environment of the aortic tissue for 6 hours.
Lercanidipine is commercially available from Recordati S.p.A. (Milan; Italy) and has been described along with methods for making it and resolving it into individual enantiomers in U.S. Patent Nos. 4,705,797; 5,767,136; 4,968,832; 5,912,31; and 5,696,139.
The process for preparing lercanidipine described in U.S. Patent No. 4,705,797 involves the following scheme:
Ph Ph CH3 (1 ) pH
H3C~ ~~ + G -~ HsC
N Ph ~ N Ph Hs O O CH3 Ph i~~ H
CH3 O ~N -~ (s) N02 CH3 Ph ~ \ p- N~~.~Ph +
I Hs ~3 ~3 O CHs (4) Lercanidipine (1 ): xylene at reflux; (2): toluene, 85°C; (3) HCI +CHCI3; 0°C;
(4) HO-CH(CH3)2 at reflux The crude lercanidipine is an oily residue that must be purified by flash chromatography using chloroform; containing increasing amounts of acetone, as the eluent. The solvent is then evaporated to dryness and remaining residue is dissolved in methanol adding a small excess of hydrochloric acid in ethanol. After evaporation of the solvent; the hemi-hydrated hydrochloride salt is prepared by treatment with diluted hydrochloric acid in the presence of sodium chloride.
A major disadvantage of the process of preparing lercanidipine, as it is described in U.S.
Patent No. 4,705,797, is that the disclosed cyclization reaction generates several by-products, which results in a lower yield for the desired product. Moreover, the purification and isolation of lercanidipine from the reaction mixture is quite complex, since it requires numerous treatments with different solvents. Finally, the purification and isolation steps are difficult to perform on an industrial scale because of the necessity of purifying the product by column chromatography:
U.S. Patent 5;912,351 describes a simpler process for the preparation of lercanidipine hydrochloride. It involves reaction of 1,4-dihydro-2,6-dimethyl-5-methoxycarbonyl-4- (3-nitrophenyl) pyridine-3-carboxylic acid with thionyl chloride in dichloromethane and dimethylformamide at a temperature between -4 and +1°C and subsequent esterification of the obtained acid chloride with 2, N-dimethyl-N-(3,3-diphenylpropyl)-1-amino-2-propyl alcohol at a temperature between -10 and 0°C. The process yields lercanidipine hydrochloride in an anhydrous non-hygroscopic crystalline form, and avoids the formation of unwanted by-products and the subsequent purification on chromatography columns.
However; the isolation of lercanidipine hydrochloride in crystalline form is again quite complex. After evaporating the solvent from the reaction mixture and dissolving the residue thus obtained in ethyl aceate, the solution is washed first with brine, then washed further five times with a 10% solution of sodium carbonate, five times with 1N hydrochloric acid, and eventually once again with brine.
Therefore, there is a need in the art for a process for the preparation of lercanidipine hydrochloride in crystalline form which avoids one more of the disadvantages of the currently S used processes.
In addition, it was observed that lercanidipine, as produced by the second-described process above, displayed batch-to-batch variability despite careful process control and even observation of the melting point believed to be characteristic of the solid product obtained by the process of Example 3 of USP 5;767,136 of 186-188EC. This variability was manifest in seemingly unpredictably appearing (and disappearing} differences in one or more of product appearance (e.g., color), melting point and solubility. This raised issues as to whether assurances of purity and/or reproducibility can be made (e.g., to regulatory authorities) that the product is always the same.
Further research by the present inventors revealed bitch-to-batch differences in bioavailability in; animals, and differences in crystal size. In the course of researching the causes of the variability problem, the inventors surprisingly discovered novel lercanidipine polymorphs. They also discovered more suitable processes for the preparation and isolation of crystalline lercanidipine hydrochloride products from the reaction mixture. It was surprisingly determined that lercanidipine hydrochloride shows polymorphic features and crystallizes into different crystalline forms depending on the process followed and on the solvents used.
Furthermore, the isolation of each of these crystalline forms has become possible, thus decreasing the possibility of batch to batch variability of lercanidipine, which the present inventors determined was due to mixtures of different solid forms being present by the same batch and to such mixtures of different composition having the same melting point. As a result, more reproducible batches of lercanidipine more suitable for large scale manufacture and quality control became available by the present inventors.
SUMMARY OF THE INVENTION
The present invention provides novel crude forms and crystalline forms of lercanidipine hydrochloride and processes for making them.
In one embodiment, the invention provides novel crude lercanidipine hydrochloride Form (A), which has a melting point of about 150-152EC (DSC peak) and comprises about 3-4% (w/w) ethyl acetate.
In another embodiment, the invention provides novel crude lercanidipine hydrochloride Form (B) which has a melting point of about 131-135EC (I~SC peak) and comprises about 0.3-0.7% (w/w) ethyl acetate.
Methods are provided for the independent syntheses of crude lercanidipine hydrochloride Form (A) and crude lercanidipine hydrochloride Form (B), making possible to obtain each crude form in isolated form.
In a further embodiment, isolated lercanidipine hydrochloride crystalline Form (I) is provided which has the following X-ray diffraction pattern, at wavelength Ka wherein distances between peaks (D in X), relative intensity ratios (IIIo) ratios, and angles of significant peaks (2B) are:
NOVEL CRUDE AND CRYSTALLINE FORMS OF LERCANIDIPINE
HYDROCHLORIDE
FIELD OF THE INVENTION
The invention is directed to novel crude forms and crystalline forms of lercanidipine hydrochloride, and to processes for the preparation of these forms.
Pharmaceutical compositions comprising the novel crystalline forms also are contemplated.
BACKGROUND OF THE INVENTION
Lercanidipine (methyl l,l;N-trimethyl-N-(3,3-diphenylpropyl)-2-aminoethyl 1,4-dihydro-2,6-dimethyl-4-(3-nitrophenyl)pyridine-3,5-dicarboxylate) is a highly lipophilic dihydropyridine calcium antagonist with long duration of action and high vascular selectivity.
Its mechanism of antihypertensive activity is attributed to a direct relaxant effect on vascular smooth muscle; which lowers total peripheral resistance. The recommended starting dose of lercanidipine as monotherapy is 10 mg daily by oral route, with a drug titration as necessary to 20 mg daily. Lercanidipine is rapidly absorbed following oral administration with peak plasma levels occurring 2-3 ;hours following dosing. Elimination is essentially via the hepatic route.
By virtue of its high lipophilicity and high membrane coefficient, lercanidipine combines a short;plasma half life with a long duration of action. In fact, the preferential distribution of the drug into membranes of smooth muscle cells results in membrane-controlled pharmacokinetics which is characterized by a prolonged pharmacological effect.
In comparison -v to other calcium antagonists, lercanidipine is characterized by gradual onset and long-lasting duration of action despite decreasing plasma levels. In vitro studies show that isolated rat aorta response to high K+' may be attenuated by lercanidipine, even after the drug has been removed from the environment of the aortic tissue for 6 hours.
Lercanidipine is commercially available from Recordati S.p.A. (Milan; Italy) and has been described along with methods for making it and resolving it into individual enantiomers in U.S. Patent Nos. 4,705,797; 5,767,136; 4,968,832; 5,912,31; and 5,696,139.
The process for preparing lercanidipine described in U.S. Patent No. 4,705,797 involves the following scheme:
Ph Ph CH3 (1 ) pH
H3C~ ~~ + G -~ HsC
N Ph ~ N Ph Hs O O CH3 Ph i~~ H
CH3 O ~N -~ (s) N02 CH3 Ph ~ \ p- N~~.~Ph +
I Hs ~3 ~3 O CHs (4) Lercanidipine (1 ): xylene at reflux; (2): toluene, 85°C; (3) HCI +CHCI3; 0°C;
(4) HO-CH(CH3)2 at reflux The crude lercanidipine is an oily residue that must be purified by flash chromatography using chloroform; containing increasing amounts of acetone, as the eluent. The solvent is then evaporated to dryness and remaining residue is dissolved in methanol adding a small excess of hydrochloric acid in ethanol. After evaporation of the solvent; the hemi-hydrated hydrochloride salt is prepared by treatment with diluted hydrochloric acid in the presence of sodium chloride.
A major disadvantage of the process of preparing lercanidipine, as it is described in U.S.
Patent No. 4,705,797, is that the disclosed cyclization reaction generates several by-products, which results in a lower yield for the desired product. Moreover, the purification and isolation of lercanidipine from the reaction mixture is quite complex, since it requires numerous treatments with different solvents. Finally, the purification and isolation steps are difficult to perform on an industrial scale because of the necessity of purifying the product by column chromatography:
U.S. Patent 5;912,351 describes a simpler process for the preparation of lercanidipine hydrochloride. It involves reaction of 1,4-dihydro-2,6-dimethyl-5-methoxycarbonyl-4- (3-nitrophenyl) pyridine-3-carboxylic acid with thionyl chloride in dichloromethane and dimethylformamide at a temperature between -4 and +1°C and subsequent esterification of the obtained acid chloride with 2, N-dimethyl-N-(3,3-diphenylpropyl)-1-amino-2-propyl alcohol at a temperature between -10 and 0°C. The process yields lercanidipine hydrochloride in an anhydrous non-hygroscopic crystalline form, and avoids the formation of unwanted by-products and the subsequent purification on chromatography columns.
However; the isolation of lercanidipine hydrochloride in crystalline form is again quite complex. After evaporating the solvent from the reaction mixture and dissolving the residue thus obtained in ethyl aceate, the solution is washed first with brine, then washed further five times with a 10% solution of sodium carbonate, five times with 1N hydrochloric acid, and eventually once again with brine.
Therefore, there is a need in the art for a process for the preparation of lercanidipine hydrochloride in crystalline form which avoids one more of the disadvantages of the currently S used processes.
In addition, it was observed that lercanidipine, as produced by the second-described process above, displayed batch-to-batch variability despite careful process control and even observation of the melting point believed to be characteristic of the solid product obtained by the process of Example 3 of USP 5;767,136 of 186-188EC. This variability was manifest in seemingly unpredictably appearing (and disappearing} differences in one or more of product appearance (e.g., color), melting point and solubility. This raised issues as to whether assurances of purity and/or reproducibility can be made (e.g., to regulatory authorities) that the product is always the same.
Further research by the present inventors revealed bitch-to-batch differences in bioavailability in; animals, and differences in crystal size. In the course of researching the causes of the variability problem, the inventors surprisingly discovered novel lercanidipine polymorphs. They also discovered more suitable processes for the preparation and isolation of crystalline lercanidipine hydrochloride products from the reaction mixture. It was surprisingly determined that lercanidipine hydrochloride shows polymorphic features and crystallizes into different crystalline forms depending on the process followed and on the solvents used.
Furthermore, the isolation of each of these crystalline forms has become possible, thus decreasing the possibility of batch to batch variability of lercanidipine, which the present inventors determined was due to mixtures of different solid forms being present by the same batch and to such mixtures of different composition having the same melting point. As a result, more reproducible batches of lercanidipine more suitable for large scale manufacture and quality control became available by the present inventors.
SUMMARY OF THE INVENTION
The present invention provides novel crude forms and crystalline forms of lercanidipine hydrochloride and processes for making them.
In one embodiment, the invention provides novel crude lercanidipine hydrochloride Form (A), which has a melting point of about 150-152EC (DSC peak) and comprises about 3-4% (w/w) ethyl acetate.
In another embodiment, the invention provides novel crude lercanidipine hydrochloride Form (B) which has a melting point of about 131-135EC (I~SC peak) and comprises about 0.3-0.7% (w/w) ethyl acetate.
Methods are provided for the independent syntheses of crude lercanidipine hydrochloride Form (A) and crude lercanidipine hydrochloride Form (B), making possible to obtain each crude form in isolated form.
In a further embodiment, isolated lercanidipine hydrochloride crystalline Form (I) is provided which has the following X-ray diffraction pattern, at wavelength Ka wherein distances between peaks (D in X), relative intensity ratios (IIIo) ratios, and angles of significant peaks (2B) are:
D (X) Relative intensity 2 B angle (I/Io) 16.3 83 5.4 6.2 47 14.2 4.78 29 18:6 4.10 63 21.7 4.06 36 21.9 3.90 100 22.8 The lercanidipine hydrochloride crystalline Form (I) has a melting point of about 197-201EC, when said melting point is determined as DSC peak.
In an alternative embodiment, isolated lercanidipine hydrochloride crystalline Form (II) is provided, which has the following X-ray diffraction pattern, at wavelength Ka, as shown wherein distances, (I/Io) ratios, and 2 8 angles of significant peaks are:
D (X) Relative intensit 2 B an 1e I/Io) 9.3 35 9.5 6.0 45 14.7 5.49 65 16.1 4.65 52 19.1 4.27 74 20.8 3.81 41 23.4 3.77 100 23.6 3.58 44 24.8 3.54 29 25.2 The lercanidipine hydrochloride crystalline Form (II) has a melting point of about 207-21 lEC, when said melting point is determined as DSC peak.
The present invention thus permits obtaining mixtures of Form I and Form II
having a predetermined and reproducible content of each form, and optionally, also other forms of lercanidipine, such as amorphous.
Also provided are methods of syntheses in which each of isolated lercanidipine hydrochloride crystalline Form (I) and Form (II) may be obi;ained;
independently, from the starting material of lercanidipine hydrochloride crude Form (A) or crude Form (B).
Also provided are pharmaceutical compositions comprising (1) lercanidipine hydrochloride, wherein the lercanidipine hydrochloride is selected from the group consisting of lercanidipine hydrochloride crystalline Form (I), lercanidipine hydrochloride crystalline Form (II), and combinations thereof comprising a predetermined content of each form, and (2) at least one component selected from the group consisting of a pharmaceutically acceptable earner or diluent, a flavorant, a sweetener; a preservative, a dye, a binder, a suspending agent, a dispersing agent, a colorant, a disintegrant, an excipient, a lubricant, a plasticizer, and an edible oil.
In certain embodiments the aforementioned pharmaceutical compositions are provided as a dosage form comprising lercanidipine hydrochloride crystalline Form (I) and/or Form (II).
In further embodiments; the invention also provides for methods of treating a subject with arterial hypertension, the method comprising administering a therapeutically effective amount of lercanidipine hydrochloride crystalline Form (I), lercanidipine hydrochloride crystalline Form (II), or combinations thereof comprising a predetermined content of each form to a subject in need of such treatment.
In other embodiments, a method of treating or preventing atherosclerotic lesions in arteries of a subject is provided, the method comprising administering a therapeutically effective amount of lercanidipine hydrochloride crystalline Form (I), lercanidipine hydrochloride crystalline Form (II), or combinations hereof comprising a predetermined amount of each form, to a subject in need of such treatment.
These and other aspects of the present invention will be apparent to those of ordinary skill in the art in light of the present description, claims and figures.
BRIEF DESCRIPTION OF THE DRAWINGS
Figure 1 is a graph of DSC analysis carried out on crystalline Form (I), according to the working conditions described in Example 12. The ordinate indicates heat flow in mW and the abscissa temperature in °C.
Figure 2 is a graph of DSC analysis carned out on crystalline Form (II), according to the working conditions described in Example 12. The ordinate indicates heat flow in mW and the abscissa temperature in °C.
Figure 3 is a graph of the results of the thermogravimetric tests carried out on Form (I) and Form (II), respectively, as described in Example 13. The abscissa indicates temperature in °C and the ordinate indicates percent mass variation.
Figure 4 is a graph of solubility at 25°C of Forms (I) and (II) in ethanol at increasing water concentrations. The experiments are described in Example 15. The ordinate indicates solubility expressed as w/w and the abscissa % by weight of water in ethanol.
_g_ Figure 5 is a graph of solubility at 40°C of Forms (I) and (II) in ethanol at increasing water concentrations: The tests axe described in Example 15. The ordinate indicates solubility expressed as w/w and the abscissa % by weight of water in ethanol.
Figure 6 shows i3C NMR spectra in solid phase of crystalline Form (I). The signals and attributes of the corresponding carbon atoms can be found in Table 4.
Figure 7 shows 13C NMR spectra in solid phase of crystalline Form (II). The signals and attributes of the corresponding carbon atoms can be found in Table 5.
Figure 8 shows IR spectra of Form (I): The signal and corresponding attributes can be found in Table 6.
Figure 9 shows IR spectra of Form (II). The signal and corresponding attributes can be found in Table 7.
Figure 10 represents percent average concentration of lercanidipine hydrochloride in dog plasma after administration of crystalline Form (I) and of crystalline Form (II) in an amount of 3 mg/kg, in the form of a hard gelatin capsule. The ordinate indicates the mean value of concentration in plasma and the abscissa indicates time (in minutes).
Figures 11 and 12 show X-ray diffraction spectra at wavelength Ka of crystalline Forms (I) and (II), respectively. The distances (d) in X, the (I/Io) ratios and values of 28 angles of the most significant peaks can be found in Tables 1 and 2 below. The ordinate indicates the number of counts/sec and the abscissa shows the values of 2B angles.
Figures 13 and l4 are plots of percent mass change as a function of tinge in hygroscopicity tests carried out on Forms (I) and (II) of lercanidipine hydrochloride, respectively. The ordinate on the Left indicates percent mass changes and the ordinate on the right percent relative humidity; the abscissa indicates time in minutes. The protocol for the hygroscopicity tests are described in Example 14.
Figures 15 and 16 show X-ray diffraction spectra at wavelength Ka of crude lercanidipine hydrochloride Form (A) and of crude lercanidipine hydrochloride Form (B), respectively.
Figures 17 and 18 show Raman spectra of crude lercanidipine hydrochloride Form {A) and of crude lercanidipine hydrochloride Form (B), respectively, where the ordinate represents Raman units and the abscissa represents wave number (cm 1).
Figures 19 and 20 show the results of the thermogravimetric analysis carried out on crude lercanidipine hydrochloride Form (A) and on crude lercanidipine hydrochloride Form (B), respectively. In these figures, the abscissa indicates temperature (in °C) and the ordinate indicates percent mass variation.
DETAILED DESCRIPTION OF THE INVENTION
The present invention discloses novel crude forms and crystalline forms of lercanidipine hydrochloride and processes for making them. Applicants have determined that lercanidipine hydrochloride exhibits polymorphism and crystallizes in different forms depending on the process followed and on the solvents used, especially for crystallization.
Additionally, the various novel forms have distinct chemical and physical properties and bioavailability profiles in animals, though not in man, as discussed herein.
The novel methods for preparation of crude of lercarudipine hydrochloride are suitable for highly reproducible commercial scale production of reproducible solid compositions of lercanidipine hydrochloride. The methods advantageously produce novel crude Forms (A) and (B) of lercanidipine hydrochloride which also exhibit characteristics desirable for industrial applications. Crude Forms (A) and (B), e:g., exhibit higher solubility and faster drying rates compared to other crude forms of lercanidipine hydrochloride that have previously been reported. Crude Forms (A) and (B) further allow simplified crystallization procedures to be used for production of novel isolated crystalline forms of lereanidipine hydrochloride.
The novel isolated crystalline forms of Iercanidipine hydrochloride of the present invention can be obtained from lercanidipine hydrochloride crude Forms (A) and (B) and are termed lercanidipine hydrochloride crystalline Form (I) and Form (I17. Either of isolated Form (I) or isolated Form (II) may be reproducibly obtained from the (A) and (B) intermediates by varying the crystallization conditions as described below. Both lercanidipine hydrochloride crystalline Forms (I) and (II) exhibit good stability. Form (I) is characterized by a paler yellow color, smaller crystal size, higher solubility in aqueous meda.a (all compared to Form (In), and a melting point (DSC peak) within the rage of about 197EC to about 201EC, more specifically, 1 S about 198.7EC, and the X-ray diffraction pattern set forth, supra.
Form (In is characterized by a more pronounced yellow color, larger crystal size, slightly lower solubility in aqueous media (all compared to Form (I)), and a melting point (DSC
peak) within the range of about 207-2l lEC, more specifically about 209.3EC.
Both Form (1~ and Form (II) are stable. Form II exhibited higher bioavailability in the dog, but in man there is no difference in bioavailability between Form (I) and Form (II).
The novel crystalline Forms (1) and (II) represent crystalline forms of lercanidipine hydrochloride of a purity and uniformity that has not been obtained with previously achieved solid forms of lercanidipine hydrochloride. The purity and uniformity of Forms (I) and (II) allow for increased ease in production of lercanidipine dosage forms, due to, e.g., more precisely defined physico-chemical characteristics, such as, for example, increased uniformity of particle size following micronization and more reproducible solubility.
Forms (I) and (II) also provide dosage forms with more precisely defined characteristics, e.g.;
bioavailability, compared to previously achieved dosage formswhich the present inventors have found comprised undefined and variable mixtures of lercanidipine hydrochloride solid forms that vaxy in their physico-chemical characteristics. Finally, the availability of pure Forms (I) and (II) provides for the ability to blend the two polymorphs into dosage forms with novel controlled characteristics, e.g., a dosage form with both a rapid onset and sustained biological action.
As used herein, the term "crude form" refers to precipitated solid forms comprising crystals of a compound that have not been washed and/or recrystallized to remove impurities (including but not limited to solvent) hat may be present. In the present specification, the crude forms are referred to as Forms (A) and (B) of lercanidipine hydrochloride.
As used herein, the term "crystalline form" refers to crystals of a compound that have been washed and recrystallized to remove impurities: In the present invention;
the term crystalline forms refers to Forms (I) and (i1) of lercanidipine hydrochloride.
These crystalline forms have an HPLC purity ~ 99.5 % and residual solvents content of < 3000 ppm.
As used herein, the term "polymorphism" refers to a property of a compound to crystallize in two or more forms with distinct structures. The different crystalline forms can be detected directly by crystallographic techniques or indirectly by assessment of differences in physical and/or chemical properties associated with each particular polymorph.
The present invention contemplates any method that may be used to produce the novel crude forms of lercanidipine hydrochloride described herein. These forms have different physico-chemical properties, e:g., melting points (which can be determined byDSC analysis);
than the crude form,of lercanidipine hydrochloride produced by other known methods, e.g., by the method described in U.S. Patent No. 5,912,351; termed Form (C). Form (A) has a melting point of about 150EC to about 152EC (DSC peak), Form (13) has a melting point of about 131EC to about 135EC (DSC peak), and Form (C) has a melting point of about 186EC to about 192EC (DSC peak). Additionally, thermogravimetric studies show that Form (A) comprises 3 -4 % residual ethyl acetate and Form (B) comprises 0.3-0.7 % residual ethyl acetate, byweight.
Comparatively, the residual liquid present in Form (C) has been determined to be 0-0.1%.
The invention is directed to processes for the preparation of lercanidipine hydrochloride, each resulting in a different crude form of the product. The first two steps in producing either crude form are identical and are:
(a) reacting 2, 6-dimethyl-5-methoxycarbonyl-4-(3-nitrophenyl)-1;4-dihydropyridine-3-carboxylic acid with thionyl chloride or oxalyl chloride in a mixture of an aprotic Bipolar solvent and of an aprotic polar solvent to yield a chloride compound, and (b) in-situ reacting the chloride obtained from the above step with 2, N-dimethyl-N-(3,3-diphenylpropyl)-1-amino-2-propyl alcohol, at a temperature preferably between -5 and +5°C, in a mixture of an aprotic Bipolar solvent and of an aprotic polar solvent.
In a preferred embodiment, the mixture of an aprotic Bipolar solvent and of an aprotic polar solvent is ethyl acetate and dirnethylformamide used at a ratio of 4:1.
After the in-situ reaction, the lercanidipine hydrochloride is isolated and recovered from the mixture. The method of isolation used determines the crude form of lercanidipine hydrochloride obtained. Following the protocol below (a protocol) yields Form (A):
i) washing the mixture of step (b) preferably with water, ii) removing water from the reaction mixture of step i), preferably by azeotropic distillation under vacuum at 200-300 mmHg at a temperature below about 60°C
(preferably at 40-50°C);
iii) concentrating the mixture of step ii) preferably to about 1/3 of the initial volume at the same temperature and pressure as in step (ii), adding fresh solvent (ethyl acetate) preferably to obtain the initial volume, thus obtaining a suspension with a water content, as determined according to Karl Fischer (U.S. Pharmacopoeia 25, Method 921) preferably between 0.10 and 0.15%;
iv) cooling the suspension of step iii) preferably to 0-5°C to produce a solid;
v) filtering the solid of step iv);
vi) re-suspending the solid of step v) preferably irr ethyl acetate and stirring preferably at 60-65°C for about 1 hour; and vii) cooling to 5-10°C, filtering and drying the solid of sl;ep vi) (e.g., in an oven at about 70°C).
The second process ((3 protocol; used to prepare Forrn (B)) is performed using the following steps:
i') washing the mixture of step (b)'preferably with water, ii') removing he water from step i') preferably by azeotropically refluxing the product of step i') with a Dean Stark apparatus until a water content of about 2%, measured according to Karl Fischer, is obtained;
iii') concentrating the mixture of step ii') o preferably 3/4 of the initial volume and adding fresh solvent (ethyl acetate) to the mixture preferably until (1) the initial volume is achieved and (2) a water content, measured according to Karl Fischer, between 0.9 and 1.1 %
is obtained;
iv') cooling the solution of step iii') preferably to 0-5°C to obtain a solid;
v') filtering the solid of step iv');
vi') re-suspending the solid of step v') preferably in ethyl acetate and stirnng at preferably 60-65°C for about 1 hour; and vii') cooling the suspension of step vi') preferably to 5-10°C to produce a solid, filtering and drying the solid of step vi') preferably in an oven at about 70°C.
It is understood that these protocols are examples of methods that may be used. Any other method and obvious variations of these methods that produces Forms (A) and (B) is within the scope of the present invention.
The temperature of step vii') should be carefully controlled. The preferred range of 5-10°C is very important.
These novel crude forms of lercanidipine hydrochloride present the advantage of higher solubility and faster drying rate with regard to Form (C) and make a simplified further crystallization process possible (which can advantageously be used to prepare Form (I) or Form (II)). Compared to the crude form produced by U.S. Patent No. 5,912,351, these forms permit use of less solvent to recrystallize the compound. This increases yield by reducing loss of compound. Additionally, the methods used to produce these crude forms are more adaptable to use in a large scale setting and commercial setting.
It has been surprisingly found that crude lercanidipine hydrochloride Form (A) and Form (B), when undergoing different purification treatments, result in two novel and different crystalline forms of lercanidipine hydrochloride. Studies indicate that these novel crystalline forms have different physical and chemical properties. DSC analysis of crystalline Form (I) indicates that it has a melting peak of about I97EC to about 201EC, specifically about 198.7EC.
DSC analysis of crystalline Form (II) indicates that it has a melting temperature of about 207EC
to about 211EC, specifically about 209.3EC.
One purification process ('y process), that leads to formation of one of the novel crystalline forms ;(Form (I)) comprises the following steps:
Process for Making Form (I) d) adding isopropanol to crude lercanidipine hydrochloride (Form (A) or Form (B)) and heating under reflux with stirring to produce a solution (if the solution is not clear, it must 1 S be filtered hot);
e) cooling the solution of step d) preferably to a temperature between 30 and 40°C
and stirnng for a period of time preferably between 12 and 48 hours to produce a solid; and f) filtering the solid obtained from step e), washing the solid with isopropanol, re-filtering the solid; and drying the solid (e.g., in an oven) at preferably 70°C for a period of time preferably between 12-48 hours.
In step e), crystallization is considered complete when the content of the solution is #2% lercanidipine HCI. Other alcohols may also be used as the solvent in step d). An alternatively preferred solvent is a Cl-Cs alcohol containing a maximum of 5%
water; e.g., anhydrous ethanol. Crystalline Form (I) may be added in step (e) as seeds to further promote crystal formation;
Alternative Process for MakinE Form (I) The present application also contemplates an alternative method of producing lercanidipine hydrochloride having crystalline Form (I) which comprises the steps of d') adding ethanol to crude lercanidipine hydrochloride preferably at a weight/volume ratio of lercanidipine hydrochloride solvent of l :4 to 1:6, most preferably 1:4, refluxing under stirring in order to obtain a solution (if the solution is not clear it should preferably be filtered hot), cooling under stirring preferably to 20°C
and adding crystalline seeds of Form (I);
e') cooling the seeded mixture of step d') preferably to a temperature between and 15°C and stirring at this temperature for a period of time preferably between 24 and 96 hours to form a solid; and f ) filtering the solid of step e') and drying it preferably in an oven at preferably 70°C to obtain lercanidipine hydrochloride Form (I).
In step e'), crystallization is considered complete when the content of the solution is #
2% lercanidipine HCI. Crystalline seeds of Form (I) (preferably authentic) may also be added to steps e') to further promote crystal formation or to induce such formation.
Process for Making Form (II) The second purification process (8 process), which yields crystalline Form (II), comprises the steps of:
d") adding acetonitrile to crude lercanidipine hydrochloride (Form (A) or Form (B)) and heating the mixture under reflux and-stirring, a") cooling of the mixture of step d") to room temperature and stirring preferably for 24 hours to form a solid, f ') filtering the solid obtained from step a") and drying it preferably in an oven.
In step a"), crystallization is considered complete when the content of the solution is #
2% lercanidipine HCl The present application also contemplates two additional methods for producing Form (II).
First Alternative Process for Making Form (II) The first alternative method comprises the steps of:
d"') adding isopropanol or ethanol, preferably ethanol, with a water content preferably between 5 to 10% by weight to lercanidipine hydrochloride, refluxing with stirring to produce a solution;
a"') cooling the mixture to a temperature preferably between 20 and 40°C and stirring for a period preferably between 24 and 96 hours to form a solid;
") filtering the solid and drying (e.g:, in an oven) at preferably 70°C
for 12-l8 hours to produce lercanidipine hydrochloride Form (II).
In step a"'), crystallization is considered complete when the content of the solution is #
2% lercanidipine HCI.
Second Alternative Method for Mal~in~ Form II
The second alternative method of obtaining the Form (II) polymorph comprises the steps of d"") dissolving crude lercanidipine hydrochloride or its crystalline Form (I) in protic polar or aprotic Bipolar solvents preferably containing up to 50% by weight of water at a temperature preferably between 20 and 70°C to produce a solution;
a"") stirnng the solution of step d"") at a temperature preferably between 20 and 25°C
to produce a solid;
f"') filtering the solid of step a"") and drying (e.g., in an oven) at preferably 70°C for preferably 12-18 hours.
The second alternative method may optionally comprise the step of adding up to 60%
water to the solution of step d"") prior to step a""). The second alternative method may further comprise irradiating with ultrasound and/or adding preferably authentic crystalline seeds of Form (II) to step a""). In step a""), crystallization is considered complete when the content of the solution is #2% lercanidipine HCI. In a preferred embodiment, the erotic polar solvent is an alcohol solvent such as, but not limited to, methanol, ethanol n-propanol, isopropanol. In another preferred embodiment, the aprotic Bipolar solvent is N-methyl-pyrrolidone.
The preferred process for preparing Form (I) is the 'y processes and the preferred process for preparing Form (II) is the 8 process: Applicants have determined that Form (I) can be quantitatively obtained by use of C1-CS anhydrous alcohol (preferably anhydrous ethanol or isopropanol) or Ci-C5 alcohol containing up to 5% water under controlled conditions d' -f). In fact, the ~ and 8 processes can be used to produce the desired polymorph reproducibly and consistently.
In addition to differences in melting point, the two crystalline forms exhibit differences in x-ray structure; solubility, and bioavailability. Solubility studies show that Form (I) is more soluble than Form (II) in water, ethanol, and mixtures thereof (See Tables 2 &
3).
Bioavailability studies in dogs indicate that Form (II) is more bioavailable than Form (I) (though this difference has not been observed in man). Finally, x-ray diffraction studies show that these two forms have different diffraction patterns (see :Figures 11 and 12 and Example 20).
Form I has a smaller crystal and hence particle size before micronization and so is easier and faster to process than Form II, which presents with larger crystals.
The present application further discloses pharmaceutical formulations and unit dosage forms that comprise one of the isolated polymorphs of the present invention or a mixture thereof of predetermined,polymorph content.
The present invention is also directed to a method of treating a subject with arterial hypertension; the method comprising administering a therapeutically effective amount of isolated lercanidipine hydrochloride crystalline Form (I), lercanidipine hydrochloride crystalline Form (II), or combinations thereof of predetermined polymorph content (optionally with other form of lercanidipine, such as amorphous form) to a subject in need of such treatment.
The invention also contemplates a method of treating and preventing atherosclerotic lesions in arteries of a subject, the method comprising administering a therapeutically effective amount of isolated lercanidipine hydrochloride crystalline Form (I), isolated lercanidipine hydrochloride crystalline Form (II), or combinations thereof to a subject in need of such treatment.
Pharmaceutical Cornpositiohs The compounds and polymorphs of the present invention may be formulated into a pharmaceutical composition. The pharmaceutical composition also may include optional additives; such as a pharmaceutically acceptable earner or diluent, a flavorant; a sweetener, a preservative; a dye, a binder, a suspending agent; a dispersing agent, a colorant, a disintegrant, an excipient, a film forming agent, a lubricant, a plasticizer, an edible oil or any combination of two or more of the foregoing.
Both crystalline forms can undergo micronization, using any method known in the art.
The average size of particle produced by this method are preferably D(50%)2-8 ~.m, D(90%)<15 /am.
Suitable pharmaceutically acceptable earners or diluents include, but are not limited to, ethanol; water; glycerol; propylene glycol, aloe vera gel; allantoin;
glycerin; vitamin A and E
oils; mineral oil; PPG2 myristyl propionate; magnesium carbonate; potassium phosphate;
vegetable oil; animal oil; and solketal.
Suitable binders include, but are not limited to, starch; gelatin; natural sugars, such as glucose, sucrose and lactose; corn sweeteners; natural and synthetic gums, such as acacia, tragacanth, vegetable gum, and sodium alginate; carboxymethylcellulose;
hydroxypropylmethylcellulose; polyethylene glycol; povidorle; waxes; and the' like.
Suitable disintegrators include; but are not limited to, starch; e.g., corn starch, methyl cellulose, agar, bentonite, xanthan gum, sodium starch glycolate, crosspovidone and the like.
Suitable lubricants include, but are not limited to, sodium oleate, sodium stearate, sodium stearyl fumarate, magnesium stearate, sodium benzoate; sodium acetate, sodium chloride and the like.
A suitable suspending agent is, but is not limited to, bentonite, ethoxylated isostearyl alcohols, polyoxyethylene sorbitol and sorbitan esters, micracrystalline cellulose, aluminum metahydroxide, agar-agar and tragacanth, or mixtures of two or more of these substances, and the like.
Suitable dispersing and suspending agents include; but are not limited to, synthetic and natural gums, such as vegetable gum; tragacanth, acacia, alginate, dextran, sodium carboxymethylcellulose, methylcellulose, polyvinyl-pyrrolidone and gelatin.
Suitable film forming agents include, but are not limited to, hydroxypropylmethylcellulose, ethylcellulose and polymethacrylates.
Suitable plasticizers include, but are not limited to, polyethylene glycols of different molecular weights (e:g., 200-8000 Da) and propylene glycol.
Suitable colorants include, but are not limited to, ferric oxide(s), titanium dioxide and natural and synthetic lakes.
Suitable edible oils include, but are not limited to, cottonseed oil, sesame oil, coconut oil and peanut oil.
Examples of additional additives include; but are not limited to, sorbitol, talc, stearic acid, dicalcium phosphate and polydextrose.
Uhit Dosage Forms The pharmaceutical composition maybe formulated as unit dosage forms, such as tablets, pills, capsules, caplets; boluses; powders, granules, sterile parenteral solutions, sterile parenteral suspensions, sterile parenteral emulsions, elixirs, 'tinctures, metered aerosol or liquid sprays, drops, ampoules; autoinjector devices or suppositories. Unit dosage forms may be used for oral, parenteral, intranasal; sublingual or rectal administration; or for administration by inhalation or insufflation, transdermal patches, and a lyophilized composition. In general, any delivery of active ingredients that results in systemic availability of them can be used.
Preferably the unit dosage form is an oral dosage form, most; preferably a solid oral dosage form, therefore the preferred dosage forms are tablets, pills, caplets and capsules. However;
parenteral preparations also are preferred.
Solid unit dosage forms may be prepared by mixing the active agents ofahe present invention with a pharmaceutically acceptable carrier and any other desired additives as described above. The mixture is typically mixed until a homogeneous mixture of the active agents of the present invention and the carrier and any other desired additives is formed, i.e., until the active agents are dispersed evenly throughout the composition. In this case, the compositions can be formed as dry or moist granules.
Tablets or pills can be coated or otherwise compounded to form a unit dosage form which has delayed and/or prolonged action, such as time release and sustained release unit dosage forms. For example, the tablet or pill can comprise an inner dosage and an outer dosage component, the latter being in the form of a layer or envelope over the former. The two components can be separated by an enteric layer which serves to resist disintegration in the stomach and permits the inner component to pass intact into the duodenum or to be delayed in release.
Biodegradable polymers for controlling the release of the active agents;
include, but are not limited to, polylactic acid, polyepsilon caprolactone; polyhydroxy butyric acid, polyorthoesters, polyacetals, polydihydro-pyrans, polycyanoacrylates and cross-linked or amphipathic block copolymers of hydrogels.
For liquid dosage forms, the active substances or their physiologically acceptable salts are brought into solution, suspension or emulsion, optionally with the usually employed substances such as solubilizers, emulsifiers or other auxiliaries. Solvents for the active combinations and the corresponding physiologically acceptable salts, can include water, physiological salt solutions or alcohols, e.g: ethanol, propane-diol or glycerol. ', Additionally, sugar solutions such as glucose or mannitol solutions may be used. A mixture of the various solvents mentioned may further be used in the present invention:
A transdermal dosage form also is contemplated by the present invention.
Transdermal forms maybe a diffusion-driven transdermal system (transdermal patch) using either a fluid reservoir or a drug-in-adhesive matrix system. Other transdermal dosage forms include, but are not limited to, topical gels, lotions, ointments, transmucosal systems and devices, and iontohoretic (electrical diffusion) delivery system. Transdermal dosage forms may be used for timed release and sustained release of the active agents of the present invention.
Pharmaceutical compositions and unit dosage forms ~f the present invention for administration parenterally; and in particular by injection; typically include a pharmaceutically acceptable carrier, as described above. A preferred liquid carrier is vegetable oil. Injection may be, for example, intravenous, intrathecal, intramuscular, intraruminal, intratracheal, or subcutaneous.
The active agent also can be administered in the form of liposome delivery systems, such as small unilamellar vesicles, large unilamellar vesicles and multilamellar vesicles.
Liposomes can be formed from a variety of phospholipids, such as cholesterol;
stearylamine or phosphatidylcholines.
The polymorphs of the present invention also may be coupled with soluble polymers as targetable drug Garners. Such polymers include, but are not limited to, polyvinyl-pyrrolidone, pyran copolymer, polyhydroxypropylmethacryl-amidephenol, polyhydroxy-ethylaspartamidephenol, and polyethyl-eneoxideopolylysine substituted with palmitoyl residues.
Administration The pharmaceutical composition or unit dosage forms of the present invention maybe administered by a variety of routes such as intravenous, intratracheal, subcutaneous, oral, mucosal parenteral, buccal, sublingual, opthalmic, pulmonary, transmucosal, transdermal, and intramuscular. Unit dosage forms also can be administered i.n intranasal form via topical use of suitable intranasal vehicles, or via transdermal routes, using those forms of transdermal skin patches known to those of ordinary skill in the art. Oral adrninistration is preferred.
The pharmaceutical composition or unit dosage forms of the present invention may be administered to an animal; preferably a human being, in need of antihypertensive treatment.
The pharmaceutical composition or unit dosage form of the present invention may be administered according to a dosage and administration regimen defined by routine testing in light of the guidelines given above in order to obtain optimal antihypertensive activity and a decreased in blood pressure while minimizing toxicity or side-effects for a particular patient.
However, such fine turning of the therapeutic regimen is routine in light of the guidelines given herein.
The dosage of the composition containing polymorphs or mixtures of the present invention may vary according to a variety of factors such as underlying disease state, the individual's condition, weight; sex and age and the mode of administration.
For oral administration, the pharmaceutical compositions can be provided in the form of scored or unscored solid unit dosage forms.
A pharmaceutical composition comprising (1) lercanidipine hydrochloride, where the lercanidipine hydrochloride is selected from the group consisting of isolated lercanidipine hydrochloride crystalline Form (I), isolated lercanidipine hydrochloride crystalline Form (II), or combinations thereof of predetermined-polymorph composition; and (2) at least one component selected from the;group consisting of a pharmaceutically acceptable carrier or diluent, a flavorant, a sweetener, a preservative, a dye, a binder, a suspending agent, a dispersing agent, a colorant, a disintegrant, an excipient; a diluent, a lubricant, a plasticizer, and an edible oil. In a preferred embodiment, the pharmaceutical composition or dosage form 0.1 to 400 mg lercanidipine hydrochloride. Preferably, the composition or dosage form comprises 1 to 200 mg lercanidipine hydrochloride. More preferably, the composition or dosage form comprises S to 40 mg lercanidipine hydrochloride:
The pharmaceutical composition or unit dosage form may be administered in a single daily dose, or the total daily dosage maybe administered in divided doses. In addition, co-administration or equential administration of other active agents may be desirable. The polymorphs and mixtures thereof of the invention may be combined with any known drug therapy, preferably for treatment of hypertension. For example, bimodal therapy involving in addition a diuretic, a ~-receptor blocker, an ACE inhibitor or an angiotensin II receptor antagonist is contemplated by the present invention (see, e.g., U.S.
Provisional Application No.
60/344,601; filed October 23, 2001; Italian Application No. MI 2001 A 002136 filed October 16, 2001 ).
For combination therapy the compounds may initially be provided as separate dosage forms until an optimum dosage combination and administration regimen is achieved.
Therefore, the patient may be titrated to the appropriate dosages for his/her particular hypertensive condition. After the appropriate dosage of each of the compounds is determined to achieve a decrease of the blood pressure without untoward side effects, the patient then may be switched to a single dosage form containing the appropriate dosages of each of the active agents, or may continue with a dual dosage form.
The exact'dosage and administration regimen utilizing the combination therapy of the present invention is selected in accordance with a variety of factors including type, species, age, weight, sex and medical condition of the patient; the severity and etiology of the hypertension to be treated; the route of administration; the renal and hepatic function of the patient; the treatment history of the patient; and the responsiveness of the patient.
Optimal precision in achieving concentrations of compounds within the range that yields efficacy without toxicity requires a regimen based on the kinetics of the drug's availability to target sites. This involves a consideration of the absorption, distribution, metabolism, excretion of a drug, and responsiveness of the patient to the dosage regimen. However, such fine tuning of the therapeutic regimen is routine in light of the guidelines given herein.
A pharmaceutical composition for parenteral administration contains not below 0.1 %, preferably from about 0.5% to about 30%, by weight of a polymorph or mixture of the present invention, based upon the total weight of the pharmaceutical composition.
Individual isolated polyrnorphs are preferred for parenteral administration.
Generally; transdermal dosage forms contain from about 0.01 % to about 100% by weight of the active agents, based upon 100% total weight of the dosage.
In a preferred embodiment of the present invention, the composition is administered daily to the patient. In a further preferred embodiment, the pharmaceutical composition or 1 S dosage form 0.1 to 400 mg lercanidipine hydrochloride. Preferably, the composition or dosage form comprises l to 200 mg lercanidipine hydrochloride. More preferably, the composition or dosage form comprises 5 to 40 mg lercanidipine hydrochloride.
EXAMPLES
The following examples of preparation of lercanidipine hydrochloride crude Forms (A) and (B) and crystalline Forms (I) and (II) are now disclosed for illustrative non-limiting purposes; together with the results of DSC analysis and solubility, stability and hygroscopicity tests; the bioavailability tests for the new crystalline forms are also disclosed.
EXAMPLE 1: Initial preparation Thionyl chloride (36 g) diluted in ethyl acetate (25 g) was slowly added to a solution of 2,6-dimethyl-5-methoxycarbonyl-4-(3-nitrophenyl)-1,4-dihydropyridine-3-carboxylic acid (90 g) in dimethylformamide (11 S g) and ethyl acetate (396 g), keeping temperature between -1 and +1°C. A solution of 2, N-dimethyl-N-(3,3-diphenylpropyl)-1-amino-2-propanol (84 g) in ethyl acetate (72 g) was slowly added to the mixture thus obtained. The whole was kept under stirring at the same temperature for 3 hours. The mixture was then heated to 2U-25°C and kept under stirring for 12 hours. Water (340 ml) was then added, the whole was stirred for 30 ruin and after settling the aqueous phase was discarded. The organic phase was washed again with water (340 ml).
EXAMPLE 2- Crude lercanidipine hydrochloride Form (A) The organic phase obtained from Example 1 was than subjected to azeotropic distillation under vacuum at about 250 mmHg; without going above a temperature of 60°C. After removing about 50 ml of water, the solution was concentrated to about 1/3 of the initial volume in the same conditions of temperature and pressure and then brought to its initial volume with fresh ethyl acetate until the K.F. value (Karl Fisher value) was about 0:10-0.15%.
The final suspension was cooled to 0-5°C. The solid was filtered, suspended in ethyl acetate (350 g) and stirred at 60-65°C for 1 hour. The whole was cooled to 5-10°C
and then filtered. The solid was dried in an oven at 70°C. 133 g of dry raw lercanidipine hydrochloride Form (A) was obtained (75% yield), DSC peak 150-152°C:
EXAMPLE 3 - Crude lercanidipine hydrochloride Form (B) The organic phase obtained at the end of Example 1 was heated under reflex (70-75°C) and the water contained in the solution was removed with a Dean Stark apparatus (Spaziani Rolando, Nettuno, Rome, Italy) until a K.F. value of about 2% was obtained.
The whole was then distilled at atmospheric pressure to reach 3/4 of initial volume. The solution was brought to its initial volume by adding fresh ethyl acetate. The K.F. value at the end of this operation was 0.9-1.1 %. The final solution was cooled to 0-5°C. A solid slowly precipitates which was filtered. The solid thus obtained was suspended in ethyl acetate (350 g) and stirred at 60-65°C
for 1 hour. The whole was cooled to 5-10°C, then filtered and dried in an oven at 70°C, thus obtaining 133 g of crude lercanidipine hydrochloride Form (B), DSC peak 13 T-135°C; 75%
yield.
EXAMPLE 3A - Crude lercanidipine hydrochloride Form (B) The organic phase obtained at the end of Example 1 was heated under reflex (70-75°C) and the water contained in the solution was removed with a :Dean Stark apparatus until a K.F.
value of about 2% was obtained. The whole was then distilled at atmospheric pressure to reach 3/4 of initial volume. The solution was brought to its initial volume by adding fresh ethyl acetate. The K.F. value at the end of this operation was 0.9-1.1 %, The final solution was cooled to 20°C, seeded with 0.1 % of crude lercanidipine hydrochloride Form (B) and cooled to 0-5°C.
A solid slowly precipitated and was then filtered. The solid thus obtained was suspended in ethyl acetate (350: g);and stirred at 60-65°C for 1 hour: The whole was cooled at S-10°C, then filtered and dried in an oven at 70°C for 24 hours, thus obtaining 133 g of crude lercanidipine hydrochloride Form (B); DSC peak 131-135°C; 75% yield.
EXAMPLE 4 - Preparation of lercanidipine hydrochloride crystalline Form (I) In separate representative experiments, 100 g of crude Iercanidipine hydrochloride Form (A), (B), or (C) was loaded into a reactor, followed by 400 ml of 2-propanol.
The mixture was heated under strong reflux and under stirnng, thus obtaining an almost complete dissolution of the crude substanbe. The mixture was hot filtered to eliminate a slight opalescence and the clear solution kept under stirring was cooled to 40°C: Temperature was then set at 35°C. The whole was kept for 24 hours under stirring at 35°C, then temperature was set at 30°C, and stirring was continued at said temperature for another 24 hours. The solid was filtered at 30°C and washed with 50 rnl of 2-propanol; then dried in an oven at 70°C under vacuum for 24 hours. Weight of dry product in each case was (lercanidipine HCI (I)) 90 g (HPLC purity of the product in Form (I) > 99.5%).
EXAMPLE 4A - Preparation of lercanidipine hydrochloride crystalline Form (I) In separate representative experiments, 1U0 g of crude lercanidipine hydrochloride Form (A), (B), or (C) was loaded into a reactor, followed by 400 ml of 2-pxopanol.
The mixture was heated under strong reflux and under stirring, thus obtaining an almost complete dissolution of the crude substance. The mixture was hot filtered to eliminate a slight opalescence and the clear solution kept under stirnng is slowly cooled to 40°C. Precipitation was then triggered with 100 mg of lercanidipine hydrochloride Form (I) and temperature was set at 35°C, keeping the mixture under stirring. The whole was kept for 24 hours under stirnng at 35°C, then temperature was set at 30°C, keeping under stirring at said temperature for another 24 hours.
The solid was filtered at 30°C and washed with 50 ml of Z-propanol, then dried in an oven at 70°C under vacuum: for 24 hours. Weight of dry product (lercanidipine HCl (I)) was 90 g (HPLC purity of the product in Form (I) > 99.5%).
EXAMPLE 5- Preparation of lercanidipine hydrochloride crystalline Form (I) In independent preparations; 25 kg of crude lercanidipine hydrochloride, Form (A) or (B), and then 100 mL of 95% ethanol were loaded and brought to strong reflux under stirring.
The solution was cooled under stirring at 20°C and then seeded with crystalline Form (I). The whole was then cooled to a temperature between 10 and 15°C, keeping the reaction mixture under stirring for 4 days. The solid thus obtained was filtered and washed with 95% ethanol, the precipitate was filtered and dried in an oven under vacuum at 70°C
for 24 hours. 20.2 kg of product was obtained, corresponding to a yield of 81%; HPLC purity in Form (I) > 99.5%.
Comparable results are obtained with Form (C) as starting material.
EXAMPLE 6 - Preparation of lercanidipine hydrochloride crystalline Form (II) 100 g of crude lercanidipine hydrochloride Form (C) and then 200 ml of acetonitrile was loaded into a reactor. The mixture was heated under strong reflux and under stirring, thus obtaining a complete dissolution. The mixture was brought to 20-30°C
under slight stirring and kept at said temperature for 24 hours. The precipitate was filtered and dried in an oven at 70°C
for 24 hours. 95 g of dry product was obtained, corresponding to a 95% yield;
HPLC purity >
99.5% in lercanidipine hydrochloride Form (II). Comparable results are obtained when lercanidipine hydrochloride Form (A) or (B) is used as starting material.
EXAMPLE 7 - Preparation of lercanidipine hydrochloride crystalline Form (I17 In separate representative experiments, 100 g of crude lercanidipine hydrochloride Form (A), (B), or (C) in 200 ml of 95% ethanol was loaded into a reactor, the mixture thus obtained was heated under stirring and under strong reflux and hen cooled at 25°C always under stirring.
The solution was kept at said temperature for 24 hours under stirring. The precipitate thus obtained was then filtered and dried in an oven at 70°C for 24 hours.
90 g of Form (II), HPLC
purity > 99.5% was obtained.
EXAMPLE 7A - Preparation of lercanidipine hydrochloride crystalline Form (II) 25 g of lercanidipine HCl crude substance or Form (C) was dissolved at 60°C in 100 ml of a mixture ethanol-H20 (8:2). The whole was filtered by ~,~ravity to eliminate the possible insoluble portion and diluted with 100 ml of H20. The solution thus obtained was stirred at 25°C as such, or it was added with 0.1 g of lercanidipine hydrochloride Form (II) or it was sonicated for 6 seconds at 20 kHz and 100 Watts, always at 25°C.
Whatever the choice, after 48 hours under stirring the precipitate thus formed was collected and dried in an oven at 70°C for 24 hours; obtaining a 80-85% yield of Form (I>7: Comparable results are obtained using crude Forms (A) or (B) or lercanidipine hydrochloride crystalline Form (I) as starting material.
As an alternative, the initial clear solution is diluted with 100 ml of ethanol and seeded with lercanidipine hydrochloride Form {II) (0.1 g). After 48 hours with stirring at 25°C, 80%
yield with respect to stoichiometric lercanidipine hydrochloride Form (II) is obtained.
EXAMPLE 8 - Preparation of lercanidipine hydrochloride crystalline Form (II) in aqueous methanol In representative independent examples, 40 g of lercanidipine hydrochloride crude Form (C) or crystalline Form (I) was dissolved in 100 ml of methanol at 30°C. The whole was filtered by gravity to eliminate the possible insoluble portion and 25 ml of water was added. The solution thus obtained was stirred at 25°C as such, or was mixed with 0.1 g of lercanidipine hydrochloride Form (II), or was sonicated for 6 seconds at 20 kHz and 100 Watts, always at 25°C. Whichever the choice, after 48 hours under stirnng the precipitate thus formed was collected and dried, with yields of 80-85% with respect to stoichiometric lercanidipine hydrochloride Form (II). Comparable results are obtained using crude Form (A) or (B).
EXAMPLE 9 - Preparation of lercanidipine hydrochloride crystalline Form (II) in aqueous 1-propanol 60 g of lercanidipine HCl crude Form (C) was dissolved at 60°C in 100 ml of 1-propanol-H20 (8:2). After filtering by gravity the possible insoluble portion the solution was cooled in two hours to 25°C and stirred for 120 hours at said.
temperature, with or without sonication for 6 seconds at 20 kHz and 100 Watts: The precipitate thus formed was collected, obtaining 90% yield with respect to stoichiometric lercanidipine hydrochloride Form (II) after a drying step. Comparable results are obtained using crude Forms (A) or (B) or lercanidipine hydrochloride crystalline Form (I) as starting material.
EXAMPLE 10 - Preparation of lercanidipine hydrochloride crystalline Form (II) in aqueous 2-propanol 30 g of lercanidipine hydrochloride crude Form (C) wvas dissolved at 60°C in 100 ml of 2-propanol-H20 (8:2). After filtering by gravity the possible insoluble portion the solution was cooled in two hours to 25°C and stirred for 72 hours at said temperature, with or without sonication for 6 seconds at 20 kHz and 100 Watts. The precipitate thus formed was collected, obtaining 85% yield with respect to stoichiometric lercanidipinehydrochloride Form (II) after a drying step. The same result is obtained by stirring for 168 hours at 10°C. Comparable results are obtained using crude Forms (A) or (B) or lercanidipine hydrochloride crystalline Form (I) as starting material.
EXAMPLE 11- Preparation of lercanidipine hydrochloride crystalline Form (II) in aqueous N-methylpyrrolidone A suspension of 50 g of lercanidipine hydrochloride crude Form (C) in 30 ml of N-methylpyrrolidone/water (1:l) was stirred at 20-25°C for 12 days. The solid thus formed was collected by filtration and dried, yielding 40 g of lercanidipine hydrochloride Form (II).
Comparable results are obtained using crude Forms (A) or (B) or lercanidipine hydrochloride crystalline Form (I) as starting material.
EXAMPLE 12 - DSC analysis of lercanidipine hydrochloride crystalline Forms (I) and (II) DSC analysis measures changes that occur in a given sample with heating, wherein the changes identify transition phases. Enthalpy variations taking place in a transition phase are calculated on the basis of the area under the curve. The most common transition phases are melting and sublimation. The temperature at which transition starts, onset T, is given by the point in which the curve starts to deviate from the base line (flex point).
DSC of Form (I): 3.8 mg of Form (I) was placed in a golden pan of the apparatus Perkin Elmer DSC7. The heating speed during,the test was 10°C/min.
DSC Form (II): 4.6 mg of Form (II) was placed in a golden pan of the apparatus Perkin Elmer DSC7. The heating speed during the test was 10°C/min.
The data are shown in Figures 1 and 2 and the characteristic points of the figures are briefly summarized in the following Table 1:
Table 1.
Compound Melting T (Tpeak) Onset T [C]
[C]
Form (I) 198.7 179.8 Form (II) 209.3 169.0 Immediately after melting of Form (I) or (II) an exothermic event due to salt decomposition can be observed.
EXAMPLE 13 - Thermogravimetry A gravimetric analysis associated with an IR analysis was carned out on both crystalline Forms (I) and (II); and also on crude lercanidipine hydrochloride Form (A) and on crude lercanidipine hydrochloride Form (B), using a Netsch Thermomicrobalance 209 in combination with a spectrometer FTIR Broker Vector 22.
The tests were carried out according to the following working conditions: 2-5 mg of sample was heated in a steel crucible in nitrogen atmosphere; with a heating speed of 10°C/min.
The results obtained with crystalline Forms (I) and (II) are shown in Figure 3, from which it can be inferred that in both crystalline forms no weight loss can be observed up to their melting point (i.e., until about 190-200°C).
During degradation, which takes places as indicated above after melting, a C02 loss can be observed.
The results obtained with crude lercanidipine hydrochloride Form (A) are shown in Figure 19; where a weight loss of 3.4% can be observed in the temperature range 25-153°C.
The volatile compound has been identified by its corresponding IR spectrum and is ethyl acetate. During degradation (T > 170°C) a small amount of ethyl acetate in gas phase could be observed.
The results obtained with crude lercanidipine hydrochloride Form (B) are shown in Figure 20, where a weight loss of 0.5% in temperature range 25-153°C
can be observed. The volatile compound identified with its corresponding IR spectrum is ethyl acetate (0.4%) and water (0.1 %). During degradation (T > 170°C) a small amount of ethyl acetate in gas phase can be observed.
EXAMPLE 14 - Hygroscopicity of crystalline Forms (I) and (II) The hygroscopicity of both crystalline Forms (I) and (II) was measured with DVS
analysis by means of a water absorption analyzer (SURFACE MEASUREMENT SYSTEM, Marion, Buckinghamshire, UK) according to the following working conditions:
10-15 mg of Form (I) and (II) respectively were placed in a quartz sample-holder, placed in its turn on a microbalance, and the sample underwent humidity cycles between 0 and 95%, starting from 50% of relative humidity (25°C, relative humidity (RH):
50-95-0-95-0-50% at RH/h:5%).
The results of the tests are shown in the diagrams of Figures 13 and 14.
14-1 Results obtained with crystalline Form (1) The exposure of Form (I) to humidity in the DVS analyzer results in a mass change of +0.15% at 95% RH, and of -0.3% at 0% RH, with almost no hysteresis during mass increase and loss. These slight variations are probably due to a reversible surface absorption of water.
14-2 Results obtained with crystalline Form (II) The exposure of Form (II) to humidity in DVS causes a negligible mass variation (<
0.05%) in the whole RH range tested.
EXAMPLE 15- Solubility of crystalline Forms (I) and (II) 15.1 Solubility in water and in ethanol at room temperature The solubility at 23°C of both crystalline Forms (I) and (II) was evaluated by UV-Visible spectroscopy in bi-distilled water (at the pH value spontaneously reached by the system) and in absolute ethanol. The molar absorptivity had been previously determined in acetonitrile.
The same molar absorptivity was considered for he determination in water and in ethanol.
Solubility in water certainly depends on pH. The residual solid obtained by filtration of the suspension was immediately analyzed with Raman spectroscopy. The results are shown in the following Tables'2 and 3.
_3g_ TABLE 2. Solubility in water (about 40 mg/ml as initial condition).
Starting materialTime [min] Solubility[mg/ml]Residual material ~~I
i Form (I) 5/25/451990 0.4/0:5/0.5/0.5Form (I) Form (II) 5/25/45/990 0.2/0.2/0.3/0.3Form (II) TABLE 3. Solubility in ethanol (100 mg/ml as initial condition) Starting materialTime [min] Solubility Residual material {mg/ml]
Form (I) 15/45/120 28/27/27 Form (I) Form (II) 15/45/120 11/12/12 Form (II) Form (II) is less soluble than Form (I) in both solvents.
15.2 Solubility in-mixtures of water-ethanol at 25°C and at 40°C, with increasing water concentrations Figures 4 and 5 show solubility in water-ethanol at 25°C and at 40°C of Form (I) and of Form (II). The maximum solubility is reached for both forms, at both temperatures, when water concentration is of 20%. Also in this case the solubility of crystalline Form (I) is higher than that of crystalline Farm (II).
EXAMPLE 16: Solid phase 13C-NMR studies The high resolution 13C-NMR solid phase spectra were carried out with the Bruker, ASX300 Instrument equipped with a 7 mm Rotor accessory, using several combined techniques:
Magic angle spi~(MAS). About 300 mg of the sample was placed in the rotor spinning at 4.3 kHz around an axis oriented at the magic angle (54°
70') to the magnetic field to overcome the Bipolar bradening caused by CSA (Chemical shift Anisotropy). The experiments were conducted at room temerature.
bipolar Coupling. Since much of line broadening in 13C spectra of organic solids is due to coupling to protons, it was removed by heteronuclear decoupling (decoupling power level was almost 1 Kilowatt).
Cross polarization (CP). Cross polarization allowed carbon magnetization from larger proton magnetization via the Bipolar coupling to increase signal intensity.
Total suppression ofsidebands TOSS). TOSS was performed using spin-echoes synchronized with the rotation of the sample to cause phase alteration of the spinning sidebands, resulting-in cancellation when successive spectra were added together.
Crystalline Forms (I) and (II) show different 13C-NMR spectra in solid phase.
The signals (chemical shift ) and attribution of the corresponding carbon atoms (as numbered in the formula of lercanidipine hydrochloride shown below) are represented in the following Tables 4 and 5, respectively.
~~ \ / 31 O 13 16 2 15 ~ / 17\ 19 25 ~9~ ~4~ ~11~ 12 N 18 f"~3Cr~ 5 3 + 2 ~~ ~ ~ /~
31' 27 g~6'H/2~ O
C
Table 4. Lercanidipine hydrochloride crystalline Form (I) Chemical shift ( ; ppm) Attribution of carbon atoms 168.7; 167.7 9; l l or 1l; 9 150.1 to 120.4 2; 6 and 20 to 37 104.3;100.9 3;5o5;3 79.7 12 63.0; 60.1 (weak) 15; 17 o r 17;15 48.6 10 47.7 16 45.4 19 41.1 4 31.6 18 27.7; 26.4 13; 14 or 14; 13 19.6; 18.0 7; 8 or 8; 7 Table 5. Lercanidipine hydrochloride crystalline Form (II) Chemical shift ( ; ppm) Attribution of carbon atoms 168.1; 166.6 9; 11 or l l; 9 151.9 to 121.9 2; 6 and from 20 to 37 104.0; 102.8 3; S or 5; 3 79.0 12 66.0; 58:0 (weak) 1 S; 17 or 17;15 49.7 10 48.8 16 44.3 19 140.5 4 I 29.8 18 ~, 27.6; 23.5 13; 14 or 14; 13 19.6; 18.3 7; 8 or 8; 7 EXAMPLE 17: IR Studies The IR (infrared) spectra were recorded in KBr powder by Diffuse Reflectance Technique using a Perkin Elmer Spectrum-one instrument. IR spectra, whose wave lengths and corresponding attribution are shown in the following Tables 6 and 7, are clearly different for the new Forms (I) and (II).
Table 6. IR spectrum in KBr powder of lercanidipine hydrochloride Form (I) Wavelength (cm -1) Attribution 3186 NH stretching 3100-2800 Alkyl and phenyl stretching 2565 N'-H stretching ', 1673 C=O tretching 1525; 1348 Asymmetric and symmetric stretching of N02 group I 1405; 1386 Bending of geminal methyl groups ', 785-685 Out-of plane bending of 5 and 3 adjacent hydrogens on aromatic rings Table 7. IR spectrum in KBr powder of lercanidipine hydrochloride Form (II) Wavelength (cm'-1) Attribution 3183 NH stretching 3100-2800 Alkyl,and phenyl stretching 2684 N'~H stretching 1705;1675 C=O stretching 1526; 1350 Asymmetric and symmetric stretching of N02 group 1402; 1380 Bending of geminal methyl groups 800-680 Out-of-plane bending of 5 and 3 adjacent hydrogens on aromatic rings EXAMPLE 18: Roman Spectra A Bruker FT-Roman RFS 100 Spectrophotometer was utilized under the following typical conditions: about 10 mg sample (without anyprevious treatment), 64 scans 2 cm 1 resolution, 100 mW laser power; Ge-detector The following Tables 8 and 9 show the most significant peaks of Kaman spectra of Form (I) and Form (II), respectively.
Table 8. Kaman' pectrum of crystalline Form (I) Wave number (cm 1) Peak intensity 1'646 M
1349 Vs 73 Vs * M= moderate; S= strong, Vs =very strong Table 9. Raman pectrum of crystalline Form (II) Wave number (cW 1) Peak intensity 1647 s 1351 Vs !, 995 M
103 Vs * M= moderate; S= strong, Vs =very strong EXAMPLE 19 - Bioavailability of crystalline Forms (I) and (II) A study was carnied out on six Beagle dogs to evaluate the bioavailability of crystalline Forms (I) and (II).
The products; in micronized form, were administered orally by hard gelatin capsules filled up with the active agent, Form (I) and (II), at a dosage of 3 mg/kg, administered once in the morning of the day of the experiment.
Blood samples were taken at given times and plasma concentrations of lercanidipine were determined with a stereoselective analytical method HPLC-MS/MS, according to the following working conditions;
Lercanidipine was extracted from dog plasma by means of a liquid-liquid extraction with a mixture of n-hexane and ethyl ether. The dry residue of the organic phase was taken up with a mixture of methanol and water and a liquid-phase chromatographic separation (LC) was carried out; the two enantiomers of lercanidipine were separated on a CHIROBIOTIC V column (Vancomycin) (particle size 5 m, column size 150 x 4.6 mm (ASTEC, NJ, USA)) and were detected with a mass spectrometer (MS/MS) by using an electrospray technique.
The analytical method was validated in a concentration range between 0.1 and 20 ng/ml of plasma for both enantiomers. The method has shown to be specific with an accuracy of 15%. The average concentrations of lercanidipine in the tables represent the sum of both enantiomers.
The profiles referring to the average concentrations of lercanidipine for both forms are shown in Figure 10. The following Tables l0 and 11 show single values referring to AUC, Tmax, Cmax and to plasma concentrations.
TABLE 10. Mean values (n=5) of AUCO-t, Cmax and Tmax of lercanidipine hydrochloride (S+R) crystalline Form (I) and crystalline Form (II), in dogs; after oral administration at a dosage of 3 mg/kg.
~ 02380202 2002-04-03 Form (I) ParameterDog Dog Dog Dog Dog Dog Mean SD
2* 3- 4 5 6 AUCO-t 15:41263.8327.54446.57 70.39 28.72 37.73 19.12 ng/h/ml Tmax (h) 2:00 4:00 6.00 3.00 3:00 6.00 4.00 1.67 Cmax 8:29 128.8711.62 27:17 22.58 17:83 17.50 6.91 (ng/ml) Form (II) ParameterDog Dog 2* Dog Dog Dog Dog Mean SD
AUCO-t 54:59119.77 75.62173:82142.34 61.91 104:6843.99 nglh/ml Tmax (h) 3:00 1.50 1.50 4.00 2:00 6.00 3.00 1.61 Cmax 18:4652.19 19.78 52.64 55.38 18.56 36.17 17:27 (n~ml) * not included W the calculation of mean value Table 11: Average concentration in plasma of lercanidipine hydrochloride (S+R) crystalline Form (1) and crystalline Form (II), in dogs, after oral administration at a dosage of 3 mg/kg.
Form (I) Time Dog Dog Dog Dog Dog Dog Mean SD
(h) 1 2* 3 4 5 6 0 0.00 0.00 0.00 0.00 0.00 0.00 0:00 0:00 0.5 0.1 0.20 0.00 0:00 0.00 0.00 0.00 0.02 1 0.59 0.29 0.00 0.00 0.00 0.00 0.12 0.22 1.5 1.83 1.06 0.32 0.00 1.33 0.00 0.70 0.73 2 8.29 8.94 0:94 0.35 17.11 0.28 5.39 6.34 3 4.44 36.39 0.92 27.17 22.58 1.29 11.28 11.11 4 1:81 128:879.42 11.07 16.39 6.26 8:99 5.56 6 0.80 26.65 11.62 2.53 9.73 17.83 8.50 6.50 Form (II) Time (h) Dog 1 Dog Dog Dog Dog Dog Mean SD
2* 3 4 5 6 0 0.00 0.00 0.00 0:00 0.00 0.00 0.00 0.00 0.5 0.00 22.67 6.99 0.00 0.00 0.00 1.40 2.61 1 0:00 '52.13 16:61 5.50 3.28 0.00 5.08 5.91 1.5 0.23 52.19 19.78 35.43 32.69 3.49 18.32 14.88 2 7.63 35.45 17.81 38.10 55.38 10.19 25.82 19.23 3 18.46 17.43 15.80 28.36 40.57 14.10 23.46 12.56 4 14.83 5.17 14.10 52.64 23.66 13.24 23.69 16.26 6 8.05 4.50 3:62 17.46 6.76 18.56 10.89 6.82 * not included in the calculation of mean value The formulation containing Form (II) is more bioavailable than the one containing crystalline Form (I) in 5 animals out of 6.
To simplify the comparison, dog 2 was, excluded from the evaluation, since after the administration of Form (I) dog 2 shows a plasma AUC of 264 ng/h/ml versus a mean value of 38 19 (SD) of the other 5 dogs. On the other hand, its AUC after administration of Form (I) is similar to that of the' other animals; the value being 120 versus 105 44 ng/h/ml.
The bioavailability of lercanidipine hydrochloride (Form (II)), expressed as increase in the AUC of lercanidipine (R+S) obtained after administration of Form (II), is about 3 times S higher than that obtained with Form (I). The average profile of plasma concentrations for both crystalline forms is shown in Figure 10 The analysis of these results shows that the amount of lercanidipine (S+R) absorbed after administration of crystalline Form (II) is 3 times higher that of Form (I), whereas the absorption speed; expressed as Tmax, is practically unchanged.
Plasma concentrations 6 hours after administration (last sampling time) are similar, the concentrations being of 8:5 6.5 after administration of Form (I) and of 10.9 6.8 ng/ml after administration of'Form (II).
EXAMPLE 20 X-ray diffraction studies Philips PW 1710 and Philips X pert PW 3040 powder diffractometer (Copper Koc radiation) were used; under the following typical conditions: about 5-70 mg sample (without any previous treatment) with application of a slight pressure to obtain a flat surface. Ambient air atmosphere. 0:02° 2B stepsize; 2 sec step-1, 2-50 28.
The obtained spectra are given in Figures 11 and 12 and the corresponding main peaks are described in Tables 12 and 13. The data are clearly different for new isolated Forms (I) and (II).
Table 12. X RD spectrum of lercanidipine hydrochloride Form (I).
D, (O) Relative intensity2 B angle (I/Io) 16.3 83 5:4 6.2 47 14.2 4.78 29 18.6 4.10 63 21.7 4.06 36 21.9 3.90 100 22.8 Table 13. X RD; spectrum of lercanidipine hydrochloride Form (II).
D (0) Relative intensity2 8 angle (I/Io) 9.3 35 9.5 6.0 45 14.7 5.49 65 16:1 4.65 52 19.1 4.27 74 20.8 3.81 41 23.4 3'.77 100 23.6 3.58 44 24.8 3.54 29 25.2 EXAMPLE 21. Melting point determination of various mixtures of lercanidipine hydrochloride crystalline Forms (I) and (II) The melting points of compositions consisting of known ratios of lercanidipine hydrochloride crystalline Forms (I) and (II) were determined manually. Conditions consisted of using a set point of 177°C and introducing the capillary into the instrument (Melting Point Apparatus model 535; Biichi Labortechnik AG, Flawil; Switzerland) at approximately 5°C below the melting point. Results are shown in Table 14.
Table 14. Melting points of compositions consisting of known ratios of lercanidipine hydrochloride crystalline Forms (I) and (II) . Samples in Series A and Series B were heated at a gradient of 1 °C/min and 0.5°C/min, respectively. Results are given in °C.
Ratio lercanidipine hydrochloride crystalline Sample Pure Form Pure (n:
Form (I>) Form 9;1 7:3 1:1 3:7 1:9 Form (I) (II) Series 186.8 188.0 189.5 190.0 192.2 194.2 194.3 A
Series 185.9- 184:4- 184.5- 186.7- 186:5- 188.7- 190.6-B
186.8 186.1 187.0 187.4 189.4 190.5 192.9 U.S: Patent No. 5,767,136 discloses crystalline lercanidipine hydrochloride as having a melting point of 186-188°C. Table 14 shows that this melting point is exhibited by mixtures of Form (I) and Form(II) in which the ratio of Form (I):Form (II) varies between 9:1 to 3:7. Bianchi et al: (Drugs of the Future, 1987, 12:1113-1110 report a melting point of 186-188EC (non DSC) for a lercanidipine product they characterize as "crystals".
Hence, the melting point of a preparation of lercanidipine hydrochloride is not sufficient by itself to distinguish the particular form or forms present therein; and many mixtures of different compositions have the same melting point range.
EXAMPLE 22. Micronization of lercanidipine hydrochloride.
Micronization is carried out by a jet-mill process using a MICRONETTE H300 from the firm NUEVA GUSEO (Villanova sull'Arda -PC- Italy). Parameters are as follows:
Injection pressure, 5 Kg/cmq; micronization pressure, 9 Kg/cmq; and cyclone pressure, 2:5 Kg/cmq.
Capacity of micronization is 16 Kg/h. Particle size is determined by laser light scattering using a GALAI CIS 1 laser instrument (GALAI; Haifa, Israel). Micronization is performed to obtain an average particle size of D (S0%) 2-8 ~.m and' D (90%) < 15 ~;m.
*
The present invention is not to be limited in scope by the specific embodiments described herein. Indeed, various modifications of the invention in addition to those described herein will become apparent to those skilled in the art from the foregoing description and the accompanying figures. Such modifications are intended to fall within the scope of the appended claims.
Patents, patent applications, publications; procedures, and the like are cited throughout this application, the disclosures of which are incorporated herein by reference in their entireties.
In an alternative embodiment, isolated lercanidipine hydrochloride crystalline Form (II) is provided, which has the following X-ray diffraction pattern, at wavelength Ka, as shown wherein distances, (I/Io) ratios, and 2 8 angles of significant peaks are:
D (X) Relative intensit 2 B an 1e I/Io) 9.3 35 9.5 6.0 45 14.7 5.49 65 16.1 4.65 52 19.1 4.27 74 20.8 3.81 41 23.4 3.77 100 23.6 3.58 44 24.8 3.54 29 25.2 The lercanidipine hydrochloride crystalline Form (II) has a melting point of about 207-21 lEC, when said melting point is determined as DSC peak.
The present invention thus permits obtaining mixtures of Form I and Form II
having a predetermined and reproducible content of each form, and optionally, also other forms of lercanidipine, such as amorphous.
Also provided are methods of syntheses in which each of isolated lercanidipine hydrochloride crystalline Form (I) and Form (II) may be obi;ained;
independently, from the starting material of lercanidipine hydrochloride crude Form (A) or crude Form (B).
Also provided are pharmaceutical compositions comprising (1) lercanidipine hydrochloride, wherein the lercanidipine hydrochloride is selected from the group consisting of lercanidipine hydrochloride crystalline Form (I), lercanidipine hydrochloride crystalline Form (II), and combinations thereof comprising a predetermined content of each form, and (2) at least one component selected from the group consisting of a pharmaceutically acceptable earner or diluent, a flavorant, a sweetener; a preservative, a dye, a binder, a suspending agent, a dispersing agent, a colorant, a disintegrant, an excipient, a lubricant, a plasticizer, and an edible oil.
In certain embodiments the aforementioned pharmaceutical compositions are provided as a dosage form comprising lercanidipine hydrochloride crystalline Form (I) and/or Form (II).
In further embodiments; the invention also provides for methods of treating a subject with arterial hypertension, the method comprising administering a therapeutically effective amount of lercanidipine hydrochloride crystalline Form (I), lercanidipine hydrochloride crystalline Form (II), or combinations thereof comprising a predetermined content of each form to a subject in need of such treatment.
In other embodiments, a method of treating or preventing atherosclerotic lesions in arteries of a subject is provided, the method comprising administering a therapeutically effective amount of lercanidipine hydrochloride crystalline Form (I), lercanidipine hydrochloride crystalline Form (II), or combinations hereof comprising a predetermined amount of each form, to a subject in need of such treatment.
These and other aspects of the present invention will be apparent to those of ordinary skill in the art in light of the present description, claims and figures.
BRIEF DESCRIPTION OF THE DRAWINGS
Figure 1 is a graph of DSC analysis carried out on crystalline Form (I), according to the working conditions described in Example 12. The ordinate indicates heat flow in mW and the abscissa temperature in °C.
Figure 2 is a graph of DSC analysis carned out on crystalline Form (II), according to the working conditions described in Example 12. The ordinate indicates heat flow in mW and the abscissa temperature in °C.
Figure 3 is a graph of the results of the thermogravimetric tests carried out on Form (I) and Form (II), respectively, as described in Example 13. The abscissa indicates temperature in °C and the ordinate indicates percent mass variation.
Figure 4 is a graph of solubility at 25°C of Forms (I) and (II) in ethanol at increasing water concentrations. The experiments are described in Example 15. The ordinate indicates solubility expressed as w/w and the abscissa % by weight of water in ethanol.
_g_ Figure 5 is a graph of solubility at 40°C of Forms (I) and (II) in ethanol at increasing water concentrations: The tests axe described in Example 15. The ordinate indicates solubility expressed as w/w and the abscissa % by weight of water in ethanol.
Figure 6 shows i3C NMR spectra in solid phase of crystalline Form (I). The signals and attributes of the corresponding carbon atoms can be found in Table 4.
Figure 7 shows 13C NMR spectra in solid phase of crystalline Form (II). The signals and attributes of the corresponding carbon atoms can be found in Table 5.
Figure 8 shows IR spectra of Form (I): The signal and corresponding attributes can be found in Table 6.
Figure 9 shows IR spectra of Form (II). The signal and corresponding attributes can be found in Table 7.
Figure 10 represents percent average concentration of lercanidipine hydrochloride in dog plasma after administration of crystalline Form (I) and of crystalline Form (II) in an amount of 3 mg/kg, in the form of a hard gelatin capsule. The ordinate indicates the mean value of concentration in plasma and the abscissa indicates time (in minutes).
Figures 11 and 12 show X-ray diffraction spectra at wavelength Ka of crystalline Forms (I) and (II), respectively. The distances (d) in X, the (I/Io) ratios and values of 28 angles of the most significant peaks can be found in Tables 1 and 2 below. The ordinate indicates the number of counts/sec and the abscissa shows the values of 2B angles.
Figures 13 and l4 are plots of percent mass change as a function of tinge in hygroscopicity tests carried out on Forms (I) and (II) of lercanidipine hydrochloride, respectively. The ordinate on the Left indicates percent mass changes and the ordinate on the right percent relative humidity; the abscissa indicates time in minutes. The protocol for the hygroscopicity tests are described in Example 14.
Figures 15 and 16 show X-ray diffraction spectra at wavelength Ka of crude lercanidipine hydrochloride Form (A) and of crude lercanidipine hydrochloride Form (B), respectively.
Figures 17 and 18 show Raman spectra of crude lercanidipine hydrochloride Form {A) and of crude lercanidipine hydrochloride Form (B), respectively, where the ordinate represents Raman units and the abscissa represents wave number (cm 1).
Figures 19 and 20 show the results of the thermogravimetric analysis carried out on crude lercanidipine hydrochloride Form (A) and on crude lercanidipine hydrochloride Form (B), respectively. In these figures, the abscissa indicates temperature (in °C) and the ordinate indicates percent mass variation.
DETAILED DESCRIPTION OF THE INVENTION
The present invention discloses novel crude forms and crystalline forms of lercanidipine hydrochloride and processes for making them. Applicants have determined that lercanidipine hydrochloride exhibits polymorphism and crystallizes in different forms depending on the process followed and on the solvents used, especially for crystallization.
Additionally, the various novel forms have distinct chemical and physical properties and bioavailability profiles in animals, though not in man, as discussed herein.
The novel methods for preparation of crude of lercarudipine hydrochloride are suitable for highly reproducible commercial scale production of reproducible solid compositions of lercanidipine hydrochloride. The methods advantageously produce novel crude Forms (A) and (B) of lercanidipine hydrochloride which also exhibit characteristics desirable for industrial applications. Crude Forms (A) and (B), e:g., exhibit higher solubility and faster drying rates compared to other crude forms of lercanidipine hydrochloride that have previously been reported. Crude Forms (A) and (B) further allow simplified crystallization procedures to be used for production of novel isolated crystalline forms of lereanidipine hydrochloride.
The novel isolated crystalline forms of Iercanidipine hydrochloride of the present invention can be obtained from lercanidipine hydrochloride crude Forms (A) and (B) and are termed lercanidipine hydrochloride crystalline Form (I) and Form (I17. Either of isolated Form (I) or isolated Form (II) may be reproducibly obtained from the (A) and (B) intermediates by varying the crystallization conditions as described below. Both lercanidipine hydrochloride crystalline Forms (I) and (II) exhibit good stability. Form (I) is characterized by a paler yellow color, smaller crystal size, higher solubility in aqueous meda.a (all compared to Form (In), and a melting point (DSC peak) within the rage of about 197EC to about 201EC, more specifically, 1 S about 198.7EC, and the X-ray diffraction pattern set forth, supra.
Form (In is characterized by a more pronounced yellow color, larger crystal size, slightly lower solubility in aqueous media (all compared to Form (I)), and a melting point (DSC
peak) within the range of about 207-2l lEC, more specifically about 209.3EC.
Both Form (1~ and Form (II) are stable. Form II exhibited higher bioavailability in the dog, but in man there is no difference in bioavailability between Form (I) and Form (II).
The novel crystalline Forms (1) and (II) represent crystalline forms of lercanidipine hydrochloride of a purity and uniformity that has not been obtained with previously achieved solid forms of lercanidipine hydrochloride. The purity and uniformity of Forms (I) and (II) allow for increased ease in production of lercanidipine dosage forms, due to, e.g., more precisely defined physico-chemical characteristics, such as, for example, increased uniformity of particle size following micronization and more reproducible solubility.
Forms (I) and (II) also provide dosage forms with more precisely defined characteristics, e.g.;
bioavailability, compared to previously achieved dosage formswhich the present inventors have found comprised undefined and variable mixtures of lercanidipine hydrochloride solid forms that vaxy in their physico-chemical characteristics. Finally, the availability of pure Forms (I) and (II) provides for the ability to blend the two polymorphs into dosage forms with novel controlled characteristics, e.g., a dosage form with both a rapid onset and sustained biological action.
As used herein, the term "crude form" refers to precipitated solid forms comprising crystals of a compound that have not been washed and/or recrystallized to remove impurities (including but not limited to solvent) hat may be present. In the present specification, the crude forms are referred to as Forms (A) and (B) of lercanidipine hydrochloride.
As used herein, the term "crystalline form" refers to crystals of a compound that have been washed and recrystallized to remove impurities: In the present invention;
the term crystalline forms refers to Forms (I) and (i1) of lercanidipine hydrochloride.
These crystalline forms have an HPLC purity ~ 99.5 % and residual solvents content of < 3000 ppm.
As used herein, the term "polymorphism" refers to a property of a compound to crystallize in two or more forms with distinct structures. The different crystalline forms can be detected directly by crystallographic techniques or indirectly by assessment of differences in physical and/or chemical properties associated with each particular polymorph.
The present invention contemplates any method that may be used to produce the novel crude forms of lercanidipine hydrochloride described herein. These forms have different physico-chemical properties, e:g., melting points (which can be determined byDSC analysis);
than the crude form,of lercanidipine hydrochloride produced by other known methods, e.g., by the method described in U.S. Patent No. 5,912,351; termed Form (C). Form (A) has a melting point of about 150EC to about 152EC (DSC peak), Form (13) has a melting point of about 131EC to about 135EC (DSC peak), and Form (C) has a melting point of about 186EC to about 192EC (DSC peak). Additionally, thermogravimetric studies show that Form (A) comprises 3 -4 % residual ethyl acetate and Form (B) comprises 0.3-0.7 % residual ethyl acetate, byweight.
Comparatively, the residual liquid present in Form (C) has been determined to be 0-0.1%.
The invention is directed to processes for the preparation of lercanidipine hydrochloride, each resulting in a different crude form of the product. The first two steps in producing either crude form are identical and are:
(a) reacting 2, 6-dimethyl-5-methoxycarbonyl-4-(3-nitrophenyl)-1;4-dihydropyridine-3-carboxylic acid with thionyl chloride or oxalyl chloride in a mixture of an aprotic Bipolar solvent and of an aprotic polar solvent to yield a chloride compound, and (b) in-situ reacting the chloride obtained from the above step with 2, N-dimethyl-N-(3,3-diphenylpropyl)-1-amino-2-propyl alcohol, at a temperature preferably between -5 and +5°C, in a mixture of an aprotic Bipolar solvent and of an aprotic polar solvent.
In a preferred embodiment, the mixture of an aprotic Bipolar solvent and of an aprotic polar solvent is ethyl acetate and dirnethylformamide used at a ratio of 4:1.
After the in-situ reaction, the lercanidipine hydrochloride is isolated and recovered from the mixture. The method of isolation used determines the crude form of lercanidipine hydrochloride obtained. Following the protocol below (a protocol) yields Form (A):
i) washing the mixture of step (b) preferably with water, ii) removing water from the reaction mixture of step i), preferably by azeotropic distillation under vacuum at 200-300 mmHg at a temperature below about 60°C
(preferably at 40-50°C);
iii) concentrating the mixture of step ii) preferably to about 1/3 of the initial volume at the same temperature and pressure as in step (ii), adding fresh solvent (ethyl acetate) preferably to obtain the initial volume, thus obtaining a suspension with a water content, as determined according to Karl Fischer (U.S. Pharmacopoeia 25, Method 921) preferably between 0.10 and 0.15%;
iv) cooling the suspension of step iii) preferably to 0-5°C to produce a solid;
v) filtering the solid of step iv);
vi) re-suspending the solid of step v) preferably irr ethyl acetate and stirring preferably at 60-65°C for about 1 hour; and vii) cooling to 5-10°C, filtering and drying the solid of sl;ep vi) (e.g., in an oven at about 70°C).
The second process ((3 protocol; used to prepare Forrn (B)) is performed using the following steps:
i') washing the mixture of step (b)'preferably with water, ii') removing he water from step i') preferably by azeotropically refluxing the product of step i') with a Dean Stark apparatus until a water content of about 2%, measured according to Karl Fischer, is obtained;
iii') concentrating the mixture of step ii') o preferably 3/4 of the initial volume and adding fresh solvent (ethyl acetate) to the mixture preferably until (1) the initial volume is achieved and (2) a water content, measured according to Karl Fischer, between 0.9 and 1.1 %
is obtained;
iv') cooling the solution of step iii') preferably to 0-5°C to obtain a solid;
v') filtering the solid of step iv');
vi') re-suspending the solid of step v') preferably in ethyl acetate and stirnng at preferably 60-65°C for about 1 hour; and vii') cooling the suspension of step vi') preferably to 5-10°C to produce a solid, filtering and drying the solid of step vi') preferably in an oven at about 70°C.
It is understood that these protocols are examples of methods that may be used. Any other method and obvious variations of these methods that produces Forms (A) and (B) is within the scope of the present invention.
The temperature of step vii') should be carefully controlled. The preferred range of 5-10°C is very important.
These novel crude forms of lercanidipine hydrochloride present the advantage of higher solubility and faster drying rate with regard to Form (C) and make a simplified further crystallization process possible (which can advantageously be used to prepare Form (I) or Form (II)). Compared to the crude form produced by U.S. Patent No. 5,912,351, these forms permit use of less solvent to recrystallize the compound. This increases yield by reducing loss of compound. Additionally, the methods used to produce these crude forms are more adaptable to use in a large scale setting and commercial setting.
It has been surprisingly found that crude lercanidipine hydrochloride Form (A) and Form (B), when undergoing different purification treatments, result in two novel and different crystalline forms of lercanidipine hydrochloride. Studies indicate that these novel crystalline forms have different physical and chemical properties. DSC analysis of crystalline Form (I) indicates that it has a melting peak of about I97EC to about 201EC, specifically about 198.7EC.
DSC analysis of crystalline Form (II) indicates that it has a melting temperature of about 207EC
to about 211EC, specifically about 209.3EC.
One purification process ('y process), that leads to formation of one of the novel crystalline forms ;(Form (I)) comprises the following steps:
Process for Making Form (I) d) adding isopropanol to crude lercanidipine hydrochloride (Form (A) or Form (B)) and heating under reflux with stirring to produce a solution (if the solution is not clear, it must 1 S be filtered hot);
e) cooling the solution of step d) preferably to a temperature between 30 and 40°C
and stirnng for a period of time preferably between 12 and 48 hours to produce a solid; and f) filtering the solid obtained from step e), washing the solid with isopropanol, re-filtering the solid; and drying the solid (e.g., in an oven) at preferably 70°C for a period of time preferably between 12-48 hours.
In step e), crystallization is considered complete when the content of the solution is #2% lercanidipine HCI. Other alcohols may also be used as the solvent in step d). An alternatively preferred solvent is a Cl-Cs alcohol containing a maximum of 5%
water; e.g., anhydrous ethanol. Crystalline Form (I) may be added in step (e) as seeds to further promote crystal formation;
Alternative Process for MakinE Form (I) The present application also contemplates an alternative method of producing lercanidipine hydrochloride having crystalline Form (I) which comprises the steps of d') adding ethanol to crude lercanidipine hydrochloride preferably at a weight/volume ratio of lercanidipine hydrochloride solvent of l :4 to 1:6, most preferably 1:4, refluxing under stirring in order to obtain a solution (if the solution is not clear it should preferably be filtered hot), cooling under stirring preferably to 20°C
and adding crystalline seeds of Form (I);
e') cooling the seeded mixture of step d') preferably to a temperature between and 15°C and stirring at this temperature for a period of time preferably between 24 and 96 hours to form a solid; and f ) filtering the solid of step e') and drying it preferably in an oven at preferably 70°C to obtain lercanidipine hydrochloride Form (I).
In step e'), crystallization is considered complete when the content of the solution is #
2% lercanidipine HCI. Crystalline seeds of Form (I) (preferably authentic) may also be added to steps e') to further promote crystal formation or to induce such formation.
Process for Making Form (II) The second purification process (8 process), which yields crystalline Form (II), comprises the steps of:
d") adding acetonitrile to crude lercanidipine hydrochloride (Form (A) or Form (B)) and heating the mixture under reflux and-stirring, a") cooling of the mixture of step d") to room temperature and stirring preferably for 24 hours to form a solid, f ') filtering the solid obtained from step a") and drying it preferably in an oven.
In step a"), crystallization is considered complete when the content of the solution is #
2% lercanidipine HCl The present application also contemplates two additional methods for producing Form (II).
First Alternative Process for Making Form (II) The first alternative method comprises the steps of:
d"') adding isopropanol or ethanol, preferably ethanol, with a water content preferably between 5 to 10% by weight to lercanidipine hydrochloride, refluxing with stirring to produce a solution;
a"') cooling the mixture to a temperature preferably between 20 and 40°C and stirring for a period preferably between 24 and 96 hours to form a solid;
") filtering the solid and drying (e.g:, in an oven) at preferably 70°C
for 12-l8 hours to produce lercanidipine hydrochloride Form (II).
In step a"'), crystallization is considered complete when the content of the solution is #
2% lercanidipine HCI.
Second Alternative Method for Mal~in~ Form II
The second alternative method of obtaining the Form (II) polymorph comprises the steps of d"") dissolving crude lercanidipine hydrochloride or its crystalline Form (I) in protic polar or aprotic Bipolar solvents preferably containing up to 50% by weight of water at a temperature preferably between 20 and 70°C to produce a solution;
a"") stirnng the solution of step d"") at a temperature preferably between 20 and 25°C
to produce a solid;
f"') filtering the solid of step a"") and drying (e.g., in an oven) at preferably 70°C for preferably 12-18 hours.
The second alternative method may optionally comprise the step of adding up to 60%
water to the solution of step d"") prior to step a""). The second alternative method may further comprise irradiating with ultrasound and/or adding preferably authentic crystalline seeds of Form (II) to step a""). In step a""), crystallization is considered complete when the content of the solution is #2% lercanidipine HCI. In a preferred embodiment, the erotic polar solvent is an alcohol solvent such as, but not limited to, methanol, ethanol n-propanol, isopropanol. In another preferred embodiment, the aprotic Bipolar solvent is N-methyl-pyrrolidone.
The preferred process for preparing Form (I) is the 'y processes and the preferred process for preparing Form (II) is the 8 process: Applicants have determined that Form (I) can be quantitatively obtained by use of C1-CS anhydrous alcohol (preferably anhydrous ethanol or isopropanol) or Ci-C5 alcohol containing up to 5% water under controlled conditions d' -f). In fact, the ~ and 8 processes can be used to produce the desired polymorph reproducibly and consistently.
In addition to differences in melting point, the two crystalline forms exhibit differences in x-ray structure; solubility, and bioavailability. Solubility studies show that Form (I) is more soluble than Form (II) in water, ethanol, and mixtures thereof (See Tables 2 &
3).
Bioavailability studies in dogs indicate that Form (II) is more bioavailable than Form (I) (though this difference has not been observed in man). Finally, x-ray diffraction studies show that these two forms have different diffraction patterns (see :Figures 11 and 12 and Example 20).
Form I has a smaller crystal and hence particle size before micronization and so is easier and faster to process than Form II, which presents with larger crystals.
The present application further discloses pharmaceutical formulations and unit dosage forms that comprise one of the isolated polymorphs of the present invention or a mixture thereof of predetermined,polymorph content.
The present invention is also directed to a method of treating a subject with arterial hypertension; the method comprising administering a therapeutically effective amount of isolated lercanidipine hydrochloride crystalline Form (I), lercanidipine hydrochloride crystalline Form (II), or combinations thereof of predetermined polymorph content (optionally with other form of lercanidipine, such as amorphous form) to a subject in need of such treatment.
The invention also contemplates a method of treating and preventing atherosclerotic lesions in arteries of a subject, the method comprising administering a therapeutically effective amount of isolated lercanidipine hydrochloride crystalline Form (I), isolated lercanidipine hydrochloride crystalline Form (II), or combinations thereof to a subject in need of such treatment.
Pharmaceutical Cornpositiohs The compounds and polymorphs of the present invention may be formulated into a pharmaceutical composition. The pharmaceutical composition also may include optional additives; such as a pharmaceutically acceptable earner or diluent, a flavorant; a sweetener, a preservative; a dye, a binder, a suspending agent; a dispersing agent, a colorant, a disintegrant, an excipient, a film forming agent, a lubricant, a plasticizer, an edible oil or any combination of two or more of the foregoing.
Both crystalline forms can undergo micronization, using any method known in the art.
The average size of particle produced by this method are preferably D(50%)2-8 ~.m, D(90%)<15 /am.
Suitable pharmaceutically acceptable earners or diluents include, but are not limited to, ethanol; water; glycerol; propylene glycol, aloe vera gel; allantoin;
glycerin; vitamin A and E
oils; mineral oil; PPG2 myristyl propionate; magnesium carbonate; potassium phosphate;
vegetable oil; animal oil; and solketal.
Suitable binders include, but are not limited to, starch; gelatin; natural sugars, such as glucose, sucrose and lactose; corn sweeteners; natural and synthetic gums, such as acacia, tragacanth, vegetable gum, and sodium alginate; carboxymethylcellulose;
hydroxypropylmethylcellulose; polyethylene glycol; povidorle; waxes; and the' like.
Suitable disintegrators include; but are not limited to, starch; e.g., corn starch, methyl cellulose, agar, bentonite, xanthan gum, sodium starch glycolate, crosspovidone and the like.
Suitable lubricants include, but are not limited to, sodium oleate, sodium stearate, sodium stearyl fumarate, magnesium stearate, sodium benzoate; sodium acetate, sodium chloride and the like.
A suitable suspending agent is, but is not limited to, bentonite, ethoxylated isostearyl alcohols, polyoxyethylene sorbitol and sorbitan esters, micracrystalline cellulose, aluminum metahydroxide, agar-agar and tragacanth, or mixtures of two or more of these substances, and the like.
Suitable dispersing and suspending agents include; but are not limited to, synthetic and natural gums, such as vegetable gum; tragacanth, acacia, alginate, dextran, sodium carboxymethylcellulose, methylcellulose, polyvinyl-pyrrolidone and gelatin.
Suitable film forming agents include, but are not limited to, hydroxypropylmethylcellulose, ethylcellulose and polymethacrylates.
Suitable plasticizers include, but are not limited to, polyethylene glycols of different molecular weights (e:g., 200-8000 Da) and propylene glycol.
Suitable colorants include, but are not limited to, ferric oxide(s), titanium dioxide and natural and synthetic lakes.
Suitable edible oils include, but are not limited to, cottonseed oil, sesame oil, coconut oil and peanut oil.
Examples of additional additives include; but are not limited to, sorbitol, talc, stearic acid, dicalcium phosphate and polydextrose.
Uhit Dosage Forms The pharmaceutical composition maybe formulated as unit dosage forms, such as tablets, pills, capsules, caplets; boluses; powders, granules, sterile parenteral solutions, sterile parenteral suspensions, sterile parenteral emulsions, elixirs, 'tinctures, metered aerosol or liquid sprays, drops, ampoules; autoinjector devices or suppositories. Unit dosage forms may be used for oral, parenteral, intranasal; sublingual or rectal administration; or for administration by inhalation or insufflation, transdermal patches, and a lyophilized composition. In general, any delivery of active ingredients that results in systemic availability of them can be used.
Preferably the unit dosage form is an oral dosage form, most; preferably a solid oral dosage form, therefore the preferred dosage forms are tablets, pills, caplets and capsules. However;
parenteral preparations also are preferred.
Solid unit dosage forms may be prepared by mixing the active agents ofahe present invention with a pharmaceutically acceptable carrier and any other desired additives as described above. The mixture is typically mixed until a homogeneous mixture of the active agents of the present invention and the carrier and any other desired additives is formed, i.e., until the active agents are dispersed evenly throughout the composition. In this case, the compositions can be formed as dry or moist granules.
Tablets or pills can be coated or otherwise compounded to form a unit dosage form which has delayed and/or prolonged action, such as time release and sustained release unit dosage forms. For example, the tablet or pill can comprise an inner dosage and an outer dosage component, the latter being in the form of a layer or envelope over the former. The two components can be separated by an enteric layer which serves to resist disintegration in the stomach and permits the inner component to pass intact into the duodenum or to be delayed in release.
Biodegradable polymers for controlling the release of the active agents;
include, but are not limited to, polylactic acid, polyepsilon caprolactone; polyhydroxy butyric acid, polyorthoesters, polyacetals, polydihydro-pyrans, polycyanoacrylates and cross-linked or amphipathic block copolymers of hydrogels.
For liquid dosage forms, the active substances or their physiologically acceptable salts are brought into solution, suspension or emulsion, optionally with the usually employed substances such as solubilizers, emulsifiers or other auxiliaries. Solvents for the active combinations and the corresponding physiologically acceptable salts, can include water, physiological salt solutions or alcohols, e.g: ethanol, propane-diol or glycerol. ', Additionally, sugar solutions such as glucose or mannitol solutions may be used. A mixture of the various solvents mentioned may further be used in the present invention:
A transdermal dosage form also is contemplated by the present invention.
Transdermal forms maybe a diffusion-driven transdermal system (transdermal patch) using either a fluid reservoir or a drug-in-adhesive matrix system. Other transdermal dosage forms include, but are not limited to, topical gels, lotions, ointments, transmucosal systems and devices, and iontohoretic (electrical diffusion) delivery system. Transdermal dosage forms may be used for timed release and sustained release of the active agents of the present invention.
Pharmaceutical compositions and unit dosage forms ~f the present invention for administration parenterally; and in particular by injection; typically include a pharmaceutically acceptable carrier, as described above. A preferred liquid carrier is vegetable oil. Injection may be, for example, intravenous, intrathecal, intramuscular, intraruminal, intratracheal, or subcutaneous.
The active agent also can be administered in the form of liposome delivery systems, such as small unilamellar vesicles, large unilamellar vesicles and multilamellar vesicles.
Liposomes can be formed from a variety of phospholipids, such as cholesterol;
stearylamine or phosphatidylcholines.
The polymorphs of the present invention also may be coupled with soluble polymers as targetable drug Garners. Such polymers include, but are not limited to, polyvinyl-pyrrolidone, pyran copolymer, polyhydroxypropylmethacryl-amidephenol, polyhydroxy-ethylaspartamidephenol, and polyethyl-eneoxideopolylysine substituted with palmitoyl residues.
Administration The pharmaceutical composition or unit dosage forms of the present invention maybe administered by a variety of routes such as intravenous, intratracheal, subcutaneous, oral, mucosal parenteral, buccal, sublingual, opthalmic, pulmonary, transmucosal, transdermal, and intramuscular. Unit dosage forms also can be administered i.n intranasal form via topical use of suitable intranasal vehicles, or via transdermal routes, using those forms of transdermal skin patches known to those of ordinary skill in the art. Oral adrninistration is preferred.
The pharmaceutical composition or unit dosage forms of the present invention may be administered to an animal; preferably a human being, in need of antihypertensive treatment.
The pharmaceutical composition or unit dosage form of the present invention may be administered according to a dosage and administration regimen defined by routine testing in light of the guidelines given above in order to obtain optimal antihypertensive activity and a decreased in blood pressure while minimizing toxicity or side-effects for a particular patient.
However, such fine turning of the therapeutic regimen is routine in light of the guidelines given herein.
The dosage of the composition containing polymorphs or mixtures of the present invention may vary according to a variety of factors such as underlying disease state, the individual's condition, weight; sex and age and the mode of administration.
For oral administration, the pharmaceutical compositions can be provided in the form of scored or unscored solid unit dosage forms.
A pharmaceutical composition comprising (1) lercanidipine hydrochloride, where the lercanidipine hydrochloride is selected from the group consisting of isolated lercanidipine hydrochloride crystalline Form (I), isolated lercanidipine hydrochloride crystalline Form (II), or combinations thereof of predetermined-polymorph composition; and (2) at least one component selected from the;group consisting of a pharmaceutically acceptable carrier or diluent, a flavorant, a sweetener, a preservative, a dye, a binder, a suspending agent, a dispersing agent, a colorant, a disintegrant, an excipient; a diluent, a lubricant, a plasticizer, and an edible oil. In a preferred embodiment, the pharmaceutical composition or dosage form 0.1 to 400 mg lercanidipine hydrochloride. Preferably, the composition or dosage form comprises 1 to 200 mg lercanidipine hydrochloride. More preferably, the composition or dosage form comprises S to 40 mg lercanidipine hydrochloride:
The pharmaceutical composition or unit dosage form may be administered in a single daily dose, or the total daily dosage maybe administered in divided doses. In addition, co-administration or equential administration of other active agents may be desirable. The polymorphs and mixtures thereof of the invention may be combined with any known drug therapy, preferably for treatment of hypertension. For example, bimodal therapy involving in addition a diuretic, a ~-receptor blocker, an ACE inhibitor or an angiotensin II receptor antagonist is contemplated by the present invention (see, e.g., U.S.
Provisional Application No.
60/344,601; filed October 23, 2001; Italian Application No. MI 2001 A 002136 filed October 16, 2001 ).
For combination therapy the compounds may initially be provided as separate dosage forms until an optimum dosage combination and administration regimen is achieved.
Therefore, the patient may be titrated to the appropriate dosages for his/her particular hypertensive condition. After the appropriate dosage of each of the compounds is determined to achieve a decrease of the blood pressure without untoward side effects, the patient then may be switched to a single dosage form containing the appropriate dosages of each of the active agents, or may continue with a dual dosage form.
The exact'dosage and administration regimen utilizing the combination therapy of the present invention is selected in accordance with a variety of factors including type, species, age, weight, sex and medical condition of the patient; the severity and etiology of the hypertension to be treated; the route of administration; the renal and hepatic function of the patient; the treatment history of the patient; and the responsiveness of the patient.
Optimal precision in achieving concentrations of compounds within the range that yields efficacy without toxicity requires a regimen based on the kinetics of the drug's availability to target sites. This involves a consideration of the absorption, distribution, metabolism, excretion of a drug, and responsiveness of the patient to the dosage regimen. However, such fine tuning of the therapeutic regimen is routine in light of the guidelines given herein.
A pharmaceutical composition for parenteral administration contains not below 0.1 %, preferably from about 0.5% to about 30%, by weight of a polymorph or mixture of the present invention, based upon the total weight of the pharmaceutical composition.
Individual isolated polyrnorphs are preferred for parenteral administration.
Generally; transdermal dosage forms contain from about 0.01 % to about 100% by weight of the active agents, based upon 100% total weight of the dosage.
In a preferred embodiment of the present invention, the composition is administered daily to the patient. In a further preferred embodiment, the pharmaceutical composition or 1 S dosage form 0.1 to 400 mg lercanidipine hydrochloride. Preferably, the composition or dosage form comprises l to 200 mg lercanidipine hydrochloride. More preferably, the composition or dosage form comprises 5 to 40 mg lercanidipine hydrochloride.
EXAMPLES
The following examples of preparation of lercanidipine hydrochloride crude Forms (A) and (B) and crystalline Forms (I) and (II) are now disclosed for illustrative non-limiting purposes; together with the results of DSC analysis and solubility, stability and hygroscopicity tests; the bioavailability tests for the new crystalline forms are also disclosed.
EXAMPLE 1: Initial preparation Thionyl chloride (36 g) diluted in ethyl acetate (25 g) was slowly added to a solution of 2,6-dimethyl-5-methoxycarbonyl-4-(3-nitrophenyl)-1,4-dihydropyridine-3-carboxylic acid (90 g) in dimethylformamide (11 S g) and ethyl acetate (396 g), keeping temperature between -1 and +1°C. A solution of 2, N-dimethyl-N-(3,3-diphenylpropyl)-1-amino-2-propanol (84 g) in ethyl acetate (72 g) was slowly added to the mixture thus obtained. The whole was kept under stirring at the same temperature for 3 hours. The mixture was then heated to 2U-25°C and kept under stirring for 12 hours. Water (340 ml) was then added, the whole was stirred for 30 ruin and after settling the aqueous phase was discarded. The organic phase was washed again with water (340 ml).
EXAMPLE 2- Crude lercanidipine hydrochloride Form (A) The organic phase obtained from Example 1 was than subjected to azeotropic distillation under vacuum at about 250 mmHg; without going above a temperature of 60°C. After removing about 50 ml of water, the solution was concentrated to about 1/3 of the initial volume in the same conditions of temperature and pressure and then brought to its initial volume with fresh ethyl acetate until the K.F. value (Karl Fisher value) was about 0:10-0.15%.
The final suspension was cooled to 0-5°C. The solid was filtered, suspended in ethyl acetate (350 g) and stirred at 60-65°C for 1 hour. The whole was cooled to 5-10°C
and then filtered. The solid was dried in an oven at 70°C. 133 g of dry raw lercanidipine hydrochloride Form (A) was obtained (75% yield), DSC peak 150-152°C:
EXAMPLE 3 - Crude lercanidipine hydrochloride Form (B) The organic phase obtained at the end of Example 1 was heated under reflex (70-75°C) and the water contained in the solution was removed with a Dean Stark apparatus (Spaziani Rolando, Nettuno, Rome, Italy) until a K.F. value of about 2% was obtained.
The whole was then distilled at atmospheric pressure to reach 3/4 of initial volume. The solution was brought to its initial volume by adding fresh ethyl acetate. The K.F. value at the end of this operation was 0.9-1.1 %. The final solution was cooled to 0-5°C. A solid slowly precipitates which was filtered. The solid thus obtained was suspended in ethyl acetate (350 g) and stirred at 60-65°C
for 1 hour. The whole was cooled to 5-10°C, then filtered and dried in an oven at 70°C, thus obtaining 133 g of crude lercanidipine hydrochloride Form (B), DSC peak 13 T-135°C; 75%
yield.
EXAMPLE 3A - Crude lercanidipine hydrochloride Form (B) The organic phase obtained at the end of Example 1 was heated under reflex (70-75°C) and the water contained in the solution was removed with a :Dean Stark apparatus until a K.F.
value of about 2% was obtained. The whole was then distilled at atmospheric pressure to reach 3/4 of initial volume. The solution was brought to its initial volume by adding fresh ethyl acetate. The K.F. value at the end of this operation was 0.9-1.1 %, The final solution was cooled to 20°C, seeded with 0.1 % of crude lercanidipine hydrochloride Form (B) and cooled to 0-5°C.
A solid slowly precipitated and was then filtered. The solid thus obtained was suspended in ethyl acetate (350: g);and stirred at 60-65°C for 1 hour: The whole was cooled at S-10°C, then filtered and dried in an oven at 70°C for 24 hours, thus obtaining 133 g of crude lercanidipine hydrochloride Form (B); DSC peak 131-135°C; 75% yield.
EXAMPLE 4 - Preparation of lercanidipine hydrochloride crystalline Form (I) In separate representative experiments, 100 g of crude Iercanidipine hydrochloride Form (A), (B), or (C) was loaded into a reactor, followed by 400 ml of 2-propanol.
The mixture was heated under strong reflux and under stirnng, thus obtaining an almost complete dissolution of the crude substanbe. The mixture was hot filtered to eliminate a slight opalescence and the clear solution kept under stirring was cooled to 40°C: Temperature was then set at 35°C. The whole was kept for 24 hours under stirring at 35°C, then temperature was set at 30°C, and stirring was continued at said temperature for another 24 hours. The solid was filtered at 30°C and washed with 50 rnl of 2-propanol; then dried in an oven at 70°C under vacuum for 24 hours. Weight of dry product in each case was (lercanidipine HCI (I)) 90 g (HPLC purity of the product in Form (I) > 99.5%).
EXAMPLE 4A - Preparation of lercanidipine hydrochloride crystalline Form (I) In separate representative experiments, 1U0 g of crude lercanidipine hydrochloride Form (A), (B), or (C) was loaded into a reactor, followed by 400 ml of 2-pxopanol.
The mixture was heated under strong reflux and under stirring, thus obtaining an almost complete dissolution of the crude substance. The mixture was hot filtered to eliminate a slight opalescence and the clear solution kept under stirnng is slowly cooled to 40°C. Precipitation was then triggered with 100 mg of lercanidipine hydrochloride Form (I) and temperature was set at 35°C, keeping the mixture under stirring. The whole was kept for 24 hours under stirnng at 35°C, then temperature was set at 30°C, keeping under stirring at said temperature for another 24 hours.
The solid was filtered at 30°C and washed with 50 ml of Z-propanol, then dried in an oven at 70°C under vacuum: for 24 hours. Weight of dry product (lercanidipine HCl (I)) was 90 g (HPLC purity of the product in Form (I) > 99.5%).
EXAMPLE 5- Preparation of lercanidipine hydrochloride crystalline Form (I) In independent preparations; 25 kg of crude lercanidipine hydrochloride, Form (A) or (B), and then 100 mL of 95% ethanol were loaded and brought to strong reflux under stirring.
The solution was cooled under stirring at 20°C and then seeded with crystalline Form (I). The whole was then cooled to a temperature between 10 and 15°C, keeping the reaction mixture under stirring for 4 days. The solid thus obtained was filtered and washed with 95% ethanol, the precipitate was filtered and dried in an oven under vacuum at 70°C
for 24 hours. 20.2 kg of product was obtained, corresponding to a yield of 81%; HPLC purity in Form (I) > 99.5%.
Comparable results are obtained with Form (C) as starting material.
EXAMPLE 6 - Preparation of lercanidipine hydrochloride crystalline Form (II) 100 g of crude lercanidipine hydrochloride Form (C) and then 200 ml of acetonitrile was loaded into a reactor. The mixture was heated under strong reflux and under stirring, thus obtaining a complete dissolution. The mixture was brought to 20-30°C
under slight stirring and kept at said temperature for 24 hours. The precipitate was filtered and dried in an oven at 70°C
for 24 hours. 95 g of dry product was obtained, corresponding to a 95% yield;
HPLC purity >
99.5% in lercanidipine hydrochloride Form (II). Comparable results are obtained when lercanidipine hydrochloride Form (A) or (B) is used as starting material.
EXAMPLE 7 - Preparation of lercanidipine hydrochloride crystalline Form (I17 In separate representative experiments, 100 g of crude lercanidipine hydrochloride Form (A), (B), or (C) in 200 ml of 95% ethanol was loaded into a reactor, the mixture thus obtained was heated under stirring and under strong reflux and hen cooled at 25°C always under stirring.
The solution was kept at said temperature for 24 hours under stirring. The precipitate thus obtained was then filtered and dried in an oven at 70°C for 24 hours.
90 g of Form (II), HPLC
purity > 99.5% was obtained.
EXAMPLE 7A - Preparation of lercanidipine hydrochloride crystalline Form (II) 25 g of lercanidipine HCl crude substance or Form (C) was dissolved at 60°C in 100 ml of a mixture ethanol-H20 (8:2). The whole was filtered by ~,~ravity to eliminate the possible insoluble portion and diluted with 100 ml of H20. The solution thus obtained was stirred at 25°C as such, or it was added with 0.1 g of lercanidipine hydrochloride Form (II) or it was sonicated for 6 seconds at 20 kHz and 100 Watts, always at 25°C.
Whatever the choice, after 48 hours under stirring the precipitate thus formed was collected and dried in an oven at 70°C for 24 hours; obtaining a 80-85% yield of Form (I>7: Comparable results are obtained using crude Forms (A) or (B) or lercanidipine hydrochloride crystalline Form (I) as starting material.
As an alternative, the initial clear solution is diluted with 100 ml of ethanol and seeded with lercanidipine hydrochloride Form {II) (0.1 g). After 48 hours with stirring at 25°C, 80%
yield with respect to stoichiometric lercanidipine hydrochloride Form (II) is obtained.
EXAMPLE 8 - Preparation of lercanidipine hydrochloride crystalline Form (II) in aqueous methanol In representative independent examples, 40 g of lercanidipine hydrochloride crude Form (C) or crystalline Form (I) was dissolved in 100 ml of methanol at 30°C. The whole was filtered by gravity to eliminate the possible insoluble portion and 25 ml of water was added. The solution thus obtained was stirred at 25°C as such, or was mixed with 0.1 g of lercanidipine hydrochloride Form (II), or was sonicated for 6 seconds at 20 kHz and 100 Watts, always at 25°C. Whichever the choice, after 48 hours under stirnng the precipitate thus formed was collected and dried, with yields of 80-85% with respect to stoichiometric lercanidipine hydrochloride Form (II). Comparable results are obtained using crude Form (A) or (B).
EXAMPLE 9 - Preparation of lercanidipine hydrochloride crystalline Form (II) in aqueous 1-propanol 60 g of lercanidipine HCl crude Form (C) was dissolved at 60°C in 100 ml of 1-propanol-H20 (8:2). After filtering by gravity the possible insoluble portion the solution was cooled in two hours to 25°C and stirred for 120 hours at said.
temperature, with or without sonication for 6 seconds at 20 kHz and 100 Watts: The precipitate thus formed was collected, obtaining 90% yield with respect to stoichiometric lercanidipine hydrochloride Form (II) after a drying step. Comparable results are obtained using crude Forms (A) or (B) or lercanidipine hydrochloride crystalline Form (I) as starting material.
EXAMPLE 10 - Preparation of lercanidipine hydrochloride crystalline Form (II) in aqueous 2-propanol 30 g of lercanidipine hydrochloride crude Form (C) wvas dissolved at 60°C in 100 ml of 2-propanol-H20 (8:2). After filtering by gravity the possible insoluble portion the solution was cooled in two hours to 25°C and stirred for 72 hours at said temperature, with or without sonication for 6 seconds at 20 kHz and 100 Watts. The precipitate thus formed was collected, obtaining 85% yield with respect to stoichiometric lercanidipinehydrochloride Form (II) after a drying step. The same result is obtained by stirring for 168 hours at 10°C. Comparable results are obtained using crude Forms (A) or (B) or lercanidipine hydrochloride crystalline Form (I) as starting material.
EXAMPLE 11- Preparation of lercanidipine hydrochloride crystalline Form (II) in aqueous N-methylpyrrolidone A suspension of 50 g of lercanidipine hydrochloride crude Form (C) in 30 ml of N-methylpyrrolidone/water (1:l) was stirred at 20-25°C for 12 days. The solid thus formed was collected by filtration and dried, yielding 40 g of lercanidipine hydrochloride Form (II).
Comparable results are obtained using crude Forms (A) or (B) or lercanidipine hydrochloride crystalline Form (I) as starting material.
EXAMPLE 12 - DSC analysis of lercanidipine hydrochloride crystalline Forms (I) and (II) DSC analysis measures changes that occur in a given sample with heating, wherein the changes identify transition phases. Enthalpy variations taking place in a transition phase are calculated on the basis of the area under the curve. The most common transition phases are melting and sublimation. The temperature at which transition starts, onset T, is given by the point in which the curve starts to deviate from the base line (flex point).
DSC of Form (I): 3.8 mg of Form (I) was placed in a golden pan of the apparatus Perkin Elmer DSC7. The heating speed during,the test was 10°C/min.
DSC Form (II): 4.6 mg of Form (II) was placed in a golden pan of the apparatus Perkin Elmer DSC7. The heating speed during the test was 10°C/min.
The data are shown in Figures 1 and 2 and the characteristic points of the figures are briefly summarized in the following Table 1:
Table 1.
Compound Melting T (Tpeak) Onset T [C]
[C]
Form (I) 198.7 179.8 Form (II) 209.3 169.0 Immediately after melting of Form (I) or (II) an exothermic event due to salt decomposition can be observed.
EXAMPLE 13 - Thermogravimetry A gravimetric analysis associated with an IR analysis was carned out on both crystalline Forms (I) and (II); and also on crude lercanidipine hydrochloride Form (A) and on crude lercanidipine hydrochloride Form (B), using a Netsch Thermomicrobalance 209 in combination with a spectrometer FTIR Broker Vector 22.
The tests were carried out according to the following working conditions: 2-5 mg of sample was heated in a steel crucible in nitrogen atmosphere; with a heating speed of 10°C/min.
The results obtained with crystalline Forms (I) and (II) are shown in Figure 3, from which it can be inferred that in both crystalline forms no weight loss can be observed up to their melting point (i.e., until about 190-200°C).
During degradation, which takes places as indicated above after melting, a C02 loss can be observed.
The results obtained with crude lercanidipine hydrochloride Form (A) are shown in Figure 19; where a weight loss of 3.4% can be observed in the temperature range 25-153°C.
The volatile compound has been identified by its corresponding IR spectrum and is ethyl acetate. During degradation (T > 170°C) a small amount of ethyl acetate in gas phase could be observed.
The results obtained with crude lercanidipine hydrochloride Form (B) are shown in Figure 20, where a weight loss of 0.5% in temperature range 25-153°C
can be observed. The volatile compound identified with its corresponding IR spectrum is ethyl acetate (0.4%) and water (0.1 %). During degradation (T > 170°C) a small amount of ethyl acetate in gas phase can be observed.
EXAMPLE 14 - Hygroscopicity of crystalline Forms (I) and (II) The hygroscopicity of both crystalline Forms (I) and (II) was measured with DVS
analysis by means of a water absorption analyzer (SURFACE MEASUREMENT SYSTEM, Marion, Buckinghamshire, UK) according to the following working conditions:
10-15 mg of Form (I) and (II) respectively were placed in a quartz sample-holder, placed in its turn on a microbalance, and the sample underwent humidity cycles between 0 and 95%, starting from 50% of relative humidity (25°C, relative humidity (RH):
50-95-0-95-0-50% at RH/h:5%).
The results of the tests are shown in the diagrams of Figures 13 and 14.
14-1 Results obtained with crystalline Form (1) The exposure of Form (I) to humidity in the DVS analyzer results in a mass change of +0.15% at 95% RH, and of -0.3% at 0% RH, with almost no hysteresis during mass increase and loss. These slight variations are probably due to a reversible surface absorption of water.
14-2 Results obtained with crystalline Form (II) The exposure of Form (II) to humidity in DVS causes a negligible mass variation (<
0.05%) in the whole RH range tested.
EXAMPLE 15- Solubility of crystalline Forms (I) and (II) 15.1 Solubility in water and in ethanol at room temperature The solubility at 23°C of both crystalline Forms (I) and (II) was evaluated by UV-Visible spectroscopy in bi-distilled water (at the pH value spontaneously reached by the system) and in absolute ethanol. The molar absorptivity had been previously determined in acetonitrile.
The same molar absorptivity was considered for he determination in water and in ethanol.
Solubility in water certainly depends on pH. The residual solid obtained by filtration of the suspension was immediately analyzed with Raman spectroscopy. The results are shown in the following Tables'2 and 3.
_3g_ TABLE 2. Solubility in water (about 40 mg/ml as initial condition).
Starting materialTime [min] Solubility[mg/ml]Residual material ~~I
i Form (I) 5/25/451990 0.4/0:5/0.5/0.5Form (I) Form (II) 5/25/45/990 0.2/0.2/0.3/0.3Form (II) TABLE 3. Solubility in ethanol (100 mg/ml as initial condition) Starting materialTime [min] Solubility Residual material {mg/ml]
Form (I) 15/45/120 28/27/27 Form (I) Form (II) 15/45/120 11/12/12 Form (II) Form (II) is less soluble than Form (I) in both solvents.
15.2 Solubility in-mixtures of water-ethanol at 25°C and at 40°C, with increasing water concentrations Figures 4 and 5 show solubility in water-ethanol at 25°C and at 40°C of Form (I) and of Form (II). The maximum solubility is reached for both forms, at both temperatures, when water concentration is of 20%. Also in this case the solubility of crystalline Form (I) is higher than that of crystalline Farm (II).
EXAMPLE 16: Solid phase 13C-NMR studies The high resolution 13C-NMR solid phase spectra were carried out with the Bruker, ASX300 Instrument equipped with a 7 mm Rotor accessory, using several combined techniques:
Magic angle spi~(MAS). About 300 mg of the sample was placed in the rotor spinning at 4.3 kHz around an axis oriented at the magic angle (54°
70') to the magnetic field to overcome the Bipolar bradening caused by CSA (Chemical shift Anisotropy). The experiments were conducted at room temerature.
bipolar Coupling. Since much of line broadening in 13C spectra of organic solids is due to coupling to protons, it was removed by heteronuclear decoupling (decoupling power level was almost 1 Kilowatt).
Cross polarization (CP). Cross polarization allowed carbon magnetization from larger proton magnetization via the Bipolar coupling to increase signal intensity.
Total suppression ofsidebands TOSS). TOSS was performed using spin-echoes synchronized with the rotation of the sample to cause phase alteration of the spinning sidebands, resulting-in cancellation when successive spectra were added together.
Crystalline Forms (I) and (II) show different 13C-NMR spectra in solid phase.
The signals (chemical shift ) and attribution of the corresponding carbon atoms (as numbered in the formula of lercanidipine hydrochloride shown below) are represented in the following Tables 4 and 5, respectively.
~~ \ / 31 O 13 16 2 15 ~ / 17\ 19 25 ~9~ ~4~ ~11~ 12 N 18 f"~3Cr~ 5 3 + 2 ~~ ~ ~ /~
31' 27 g~6'H/2~ O
C
Table 4. Lercanidipine hydrochloride crystalline Form (I) Chemical shift ( ; ppm) Attribution of carbon atoms 168.7; 167.7 9; l l or 1l; 9 150.1 to 120.4 2; 6 and 20 to 37 104.3;100.9 3;5o5;3 79.7 12 63.0; 60.1 (weak) 15; 17 o r 17;15 48.6 10 47.7 16 45.4 19 41.1 4 31.6 18 27.7; 26.4 13; 14 or 14; 13 19.6; 18.0 7; 8 or 8; 7 Table 5. Lercanidipine hydrochloride crystalline Form (II) Chemical shift ( ; ppm) Attribution of carbon atoms 168.1; 166.6 9; 11 or l l; 9 151.9 to 121.9 2; 6 and from 20 to 37 104.0; 102.8 3; S or 5; 3 79.0 12 66.0; 58:0 (weak) 1 S; 17 or 17;15 49.7 10 48.8 16 44.3 19 140.5 4 I 29.8 18 ~, 27.6; 23.5 13; 14 or 14; 13 19.6; 18.3 7; 8 or 8; 7 EXAMPLE 17: IR Studies The IR (infrared) spectra were recorded in KBr powder by Diffuse Reflectance Technique using a Perkin Elmer Spectrum-one instrument. IR spectra, whose wave lengths and corresponding attribution are shown in the following Tables 6 and 7, are clearly different for the new Forms (I) and (II).
Table 6. IR spectrum in KBr powder of lercanidipine hydrochloride Form (I) Wavelength (cm -1) Attribution 3186 NH stretching 3100-2800 Alkyl and phenyl stretching 2565 N'-H stretching ', 1673 C=O tretching 1525; 1348 Asymmetric and symmetric stretching of N02 group I 1405; 1386 Bending of geminal methyl groups ', 785-685 Out-of plane bending of 5 and 3 adjacent hydrogens on aromatic rings Table 7. IR spectrum in KBr powder of lercanidipine hydrochloride Form (II) Wavelength (cm'-1) Attribution 3183 NH stretching 3100-2800 Alkyl,and phenyl stretching 2684 N'~H stretching 1705;1675 C=O stretching 1526; 1350 Asymmetric and symmetric stretching of N02 group 1402; 1380 Bending of geminal methyl groups 800-680 Out-of-plane bending of 5 and 3 adjacent hydrogens on aromatic rings EXAMPLE 18: Roman Spectra A Bruker FT-Roman RFS 100 Spectrophotometer was utilized under the following typical conditions: about 10 mg sample (without anyprevious treatment), 64 scans 2 cm 1 resolution, 100 mW laser power; Ge-detector The following Tables 8 and 9 show the most significant peaks of Kaman spectra of Form (I) and Form (II), respectively.
Table 8. Kaman' pectrum of crystalline Form (I) Wave number (cm 1) Peak intensity 1'646 M
1349 Vs 73 Vs * M= moderate; S= strong, Vs =very strong Table 9. Raman pectrum of crystalline Form (II) Wave number (cW 1) Peak intensity 1647 s 1351 Vs !, 995 M
103 Vs * M= moderate; S= strong, Vs =very strong EXAMPLE 19 - Bioavailability of crystalline Forms (I) and (II) A study was carnied out on six Beagle dogs to evaluate the bioavailability of crystalline Forms (I) and (II).
The products; in micronized form, were administered orally by hard gelatin capsules filled up with the active agent, Form (I) and (II), at a dosage of 3 mg/kg, administered once in the morning of the day of the experiment.
Blood samples were taken at given times and plasma concentrations of lercanidipine were determined with a stereoselective analytical method HPLC-MS/MS, according to the following working conditions;
Lercanidipine was extracted from dog plasma by means of a liquid-liquid extraction with a mixture of n-hexane and ethyl ether. The dry residue of the organic phase was taken up with a mixture of methanol and water and a liquid-phase chromatographic separation (LC) was carried out; the two enantiomers of lercanidipine were separated on a CHIROBIOTIC V column (Vancomycin) (particle size 5 m, column size 150 x 4.6 mm (ASTEC, NJ, USA)) and were detected with a mass spectrometer (MS/MS) by using an electrospray technique.
The analytical method was validated in a concentration range between 0.1 and 20 ng/ml of plasma for both enantiomers. The method has shown to be specific with an accuracy of 15%. The average concentrations of lercanidipine in the tables represent the sum of both enantiomers.
The profiles referring to the average concentrations of lercanidipine for both forms are shown in Figure 10. The following Tables l0 and 11 show single values referring to AUC, Tmax, Cmax and to plasma concentrations.
TABLE 10. Mean values (n=5) of AUCO-t, Cmax and Tmax of lercanidipine hydrochloride (S+R) crystalline Form (I) and crystalline Form (II), in dogs; after oral administration at a dosage of 3 mg/kg.
~ 02380202 2002-04-03 Form (I) ParameterDog Dog Dog Dog Dog Dog Mean SD
2* 3- 4 5 6 AUCO-t 15:41263.8327.54446.57 70.39 28.72 37.73 19.12 ng/h/ml Tmax (h) 2:00 4:00 6.00 3.00 3:00 6.00 4.00 1.67 Cmax 8:29 128.8711.62 27:17 22.58 17:83 17.50 6.91 (ng/ml) Form (II) ParameterDog Dog 2* Dog Dog Dog Dog Mean SD
AUCO-t 54:59119.77 75.62173:82142.34 61.91 104:6843.99 nglh/ml Tmax (h) 3:00 1.50 1.50 4.00 2:00 6.00 3.00 1.61 Cmax 18:4652.19 19.78 52.64 55.38 18.56 36.17 17:27 (n~ml) * not included W the calculation of mean value Table 11: Average concentration in plasma of lercanidipine hydrochloride (S+R) crystalline Form (1) and crystalline Form (II), in dogs, after oral administration at a dosage of 3 mg/kg.
Form (I) Time Dog Dog Dog Dog Dog Dog Mean SD
(h) 1 2* 3 4 5 6 0 0.00 0.00 0.00 0.00 0.00 0.00 0:00 0:00 0.5 0.1 0.20 0.00 0:00 0.00 0.00 0.00 0.02 1 0.59 0.29 0.00 0.00 0.00 0.00 0.12 0.22 1.5 1.83 1.06 0.32 0.00 1.33 0.00 0.70 0.73 2 8.29 8.94 0:94 0.35 17.11 0.28 5.39 6.34 3 4.44 36.39 0.92 27.17 22.58 1.29 11.28 11.11 4 1:81 128:879.42 11.07 16.39 6.26 8:99 5.56 6 0.80 26.65 11.62 2.53 9.73 17.83 8.50 6.50 Form (II) Time (h) Dog 1 Dog Dog Dog Dog Dog Mean SD
2* 3 4 5 6 0 0.00 0.00 0.00 0:00 0.00 0.00 0.00 0.00 0.5 0.00 22.67 6.99 0.00 0.00 0.00 1.40 2.61 1 0:00 '52.13 16:61 5.50 3.28 0.00 5.08 5.91 1.5 0.23 52.19 19.78 35.43 32.69 3.49 18.32 14.88 2 7.63 35.45 17.81 38.10 55.38 10.19 25.82 19.23 3 18.46 17.43 15.80 28.36 40.57 14.10 23.46 12.56 4 14.83 5.17 14.10 52.64 23.66 13.24 23.69 16.26 6 8.05 4.50 3:62 17.46 6.76 18.56 10.89 6.82 * not included in the calculation of mean value The formulation containing Form (II) is more bioavailable than the one containing crystalline Form (I) in 5 animals out of 6.
To simplify the comparison, dog 2 was, excluded from the evaluation, since after the administration of Form (I) dog 2 shows a plasma AUC of 264 ng/h/ml versus a mean value of 38 19 (SD) of the other 5 dogs. On the other hand, its AUC after administration of Form (I) is similar to that of the' other animals; the value being 120 versus 105 44 ng/h/ml.
The bioavailability of lercanidipine hydrochloride (Form (II)), expressed as increase in the AUC of lercanidipine (R+S) obtained after administration of Form (II), is about 3 times S higher than that obtained with Form (I). The average profile of plasma concentrations for both crystalline forms is shown in Figure 10 The analysis of these results shows that the amount of lercanidipine (S+R) absorbed after administration of crystalline Form (II) is 3 times higher that of Form (I), whereas the absorption speed; expressed as Tmax, is practically unchanged.
Plasma concentrations 6 hours after administration (last sampling time) are similar, the concentrations being of 8:5 6.5 after administration of Form (I) and of 10.9 6.8 ng/ml after administration of'Form (II).
EXAMPLE 20 X-ray diffraction studies Philips PW 1710 and Philips X pert PW 3040 powder diffractometer (Copper Koc radiation) were used; under the following typical conditions: about 5-70 mg sample (without any previous treatment) with application of a slight pressure to obtain a flat surface. Ambient air atmosphere. 0:02° 2B stepsize; 2 sec step-1, 2-50 28.
The obtained spectra are given in Figures 11 and 12 and the corresponding main peaks are described in Tables 12 and 13. The data are clearly different for new isolated Forms (I) and (II).
Table 12. X RD spectrum of lercanidipine hydrochloride Form (I).
D, (O) Relative intensity2 B angle (I/Io) 16.3 83 5:4 6.2 47 14.2 4.78 29 18.6 4.10 63 21.7 4.06 36 21.9 3.90 100 22.8 Table 13. X RD; spectrum of lercanidipine hydrochloride Form (II).
D (0) Relative intensity2 8 angle (I/Io) 9.3 35 9.5 6.0 45 14.7 5.49 65 16:1 4.65 52 19.1 4.27 74 20.8 3.81 41 23.4 3'.77 100 23.6 3.58 44 24.8 3.54 29 25.2 EXAMPLE 21. Melting point determination of various mixtures of lercanidipine hydrochloride crystalline Forms (I) and (II) The melting points of compositions consisting of known ratios of lercanidipine hydrochloride crystalline Forms (I) and (II) were determined manually. Conditions consisted of using a set point of 177°C and introducing the capillary into the instrument (Melting Point Apparatus model 535; Biichi Labortechnik AG, Flawil; Switzerland) at approximately 5°C below the melting point. Results are shown in Table 14.
Table 14. Melting points of compositions consisting of known ratios of lercanidipine hydrochloride crystalline Forms (I) and (II) . Samples in Series A and Series B were heated at a gradient of 1 °C/min and 0.5°C/min, respectively. Results are given in °C.
Ratio lercanidipine hydrochloride crystalline Sample Pure Form Pure (n:
Form (I>) Form 9;1 7:3 1:1 3:7 1:9 Form (I) (II) Series 186.8 188.0 189.5 190.0 192.2 194.2 194.3 A
Series 185.9- 184:4- 184.5- 186.7- 186:5- 188.7- 190.6-B
186.8 186.1 187.0 187.4 189.4 190.5 192.9 U.S: Patent No. 5,767,136 discloses crystalline lercanidipine hydrochloride as having a melting point of 186-188°C. Table 14 shows that this melting point is exhibited by mixtures of Form (I) and Form(II) in which the ratio of Form (I):Form (II) varies between 9:1 to 3:7. Bianchi et al: (Drugs of the Future, 1987, 12:1113-1110 report a melting point of 186-188EC (non DSC) for a lercanidipine product they characterize as "crystals".
Hence, the melting point of a preparation of lercanidipine hydrochloride is not sufficient by itself to distinguish the particular form or forms present therein; and many mixtures of different compositions have the same melting point range.
EXAMPLE 22. Micronization of lercanidipine hydrochloride.
Micronization is carried out by a jet-mill process using a MICRONETTE H300 from the firm NUEVA GUSEO (Villanova sull'Arda -PC- Italy). Parameters are as follows:
Injection pressure, 5 Kg/cmq; micronization pressure, 9 Kg/cmq; and cyclone pressure, 2:5 Kg/cmq.
Capacity of micronization is 16 Kg/h. Particle size is determined by laser light scattering using a GALAI CIS 1 laser instrument (GALAI; Haifa, Israel). Micronization is performed to obtain an average particle size of D (S0%) 2-8 ~.m and' D (90%) < 15 ~;m.
*
The present invention is not to be limited in scope by the specific embodiments described herein. Indeed, various modifications of the invention in addition to those described herein will become apparent to those skilled in the art from the foregoing description and the accompanying figures. Such modifications are intended to fall within the scope of the appended claims.
Patents, patent applications, publications; procedures, and the like are cited throughout this application, the disclosures of which are incorporated herein by reference in their entireties.
Claims (78)
1. Crude lercanidipine hydrochloride solid Form (A); having a melting point of about 150-152EC (DSC peak) and comprising about 3-4% (w/w) ethyl acetate.
2. Crude lercanidipine hydrochloride solid Form (B), having a melting point of about 131-135EC (DSC peak) and comprising about 0.3-0.7% (w/w) ethyl acetate.
3. A method of producing the crude lercanidipine hydrochloride Form of claim 1, comprising the steps of:
a) reacting 2,6-dimethyl-5-methoxycarbonyl-4-(3-nitrophenyl)-1,4-dihydropyridine-3-carboxylic acid with a chloride selected from the group consisting of thionyl chloride and oxalyl chloride in an aprotic dipolar solvent and an aprotic polar solvent to produce the corresponding carbonyl chloride;
b) reacting, in-situ, the chloride of step a) with 2, N-dimethyl-N-(3,3-diphenylpropyl)-1-amino-2-propyl alcohol to form crude lercanidipine hydrochloride; and c) isolating the crude lercanidipine hydrochloride of step b), washing the crude lercanidipine of step b) and recovering crude lercanidipine hydrochloride Form (A).
a) reacting 2,6-dimethyl-5-methoxycarbonyl-4-(3-nitrophenyl)-1,4-dihydropyridine-3-carboxylic acid with a chloride selected from the group consisting of thionyl chloride and oxalyl chloride in an aprotic dipolar solvent and an aprotic polar solvent to produce the corresponding carbonyl chloride;
b) reacting, in-situ, the chloride of step a) with 2, N-dimethyl-N-(3,3-diphenylpropyl)-1-amino-2-propyl alcohol to form crude lercanidipine hydrochloride; and c) isolating the crude lercanidipine hydrochloride of step b), washing the crude lercanidipine of step b) and recovering crude lercanidipine hydrochloride Form (A).
4. The method of claim 3 wherein the reacting step b) is conducted at a temperature between -5 and +5°C.
5. The method of claim 3 wherein step c) comprises the steps of:
i) washing the crude lercanidipine hydrochloride of step b) with water;
ii) removing the water from step i) to produce a mixture;
iii) concentrating the mixture of step ii) and adding solvent to produce a suspension having about the same volume as the initial volume of the mixture of step ii) and a water content, according to Karl Fischer, of between 0.10 and 0.15%;
iv) cooling the suspension obtained in step iii) to obtain a solid;
v) filtering the solid from step iv);
vi) re-suspending the solid of step v) in ethyl acetate;
vii) cooling the suspension of step vi) to obtain a precipitate; and viii) filtering and drying the precipitate of step vii) at about 70°C
to produce the crude lercanidipine hydrochloride Form (A).
i) washing the crude lercanidipine hydrochloride of step b) with water;
ii) removing the water from step i) to produce a mixture;
iii) concentrating the mixture of step ii) and adding solvent to produce a suspension having about the same volume as the initial volume of the mixture of step ii) and a water content, according to Karl Fischer, of between 0.10 and 0.15%;
iv) cooling the suspension obtained in step iii) to obtain a solid;
v) filtering the solid from step iv);
vi) re-suspending the solid of step v) in ethyl acetate;
vii) cooling the suspension of step vi) to obtain a precipitate; and viii) filtering and drying the precipitate of step vii) at about 70°C
to produce the crude lercanidipine hydrochloride Form (A).
6. The method of claim 3 wherein the chloride in step a) is thionyl chloride.
7. The method of claim 5 wherein step c) ii) comprises removing the water from step c) i) by azeotropic distillation under vacuum within the range 200-300 mm Hg, preferably at 250 mmHg, at a temperature no higher than 60°C, preferably within the range 40-50°C, to produce a mixture.
8. The method of claim 5 wherein the resuspending step vi) comprises stirring at 60-65°C for about 1 hour.
9. The method of claim 5 wherein the drying in step viii) is in an oven at 70°C.
10. The method of claim 5, wherein the washing step i) is with water; the mixture in step iii) is concentrated to 1/3 of its initial volume and solvent is added to produce a suspension having about the same volume as the initial volume of said mixture;
and the water content of said suspension according to Karl Fischer , is between 0.1 and 0.15%.
and the water content of said suspension according to Karl Fischer , is between 0.1 and 0.15%.
11. The method of claim 5, wherein cooling in step iv) is to a temperature within the range of 0-5BC.
12. The method of claim 5 wherein cooling in step vii) is to a temperature within range of 5-10°C.
13. A method of producing the crude lercanidipine hydrochloride Form of claim 2, comprising the steps of:
a) reacting 2,6-dimethyl-5-methoxycarbonyl-4-(3-nitrophenyl)-1,4-dihydropyridine-3-carboxylic acid with a chloride selected from the group consisting of thionyl chloride and oxalyl chloride in an aprotic dipolar solvent and an aprotic polar solvent to produce the corresponding carbonyl chloride;
b) reacting, in-situ, the chloride of step a) with 2, N-dimethyl-N-(3,3-diphenylpropyl)-1-amino-2-propyl alcohol to yield crude lercanidipine hydrochloride; and c) isolating the crude lercanidipine hydrochloride of step b), washing the crude lercanidipine hydrochloride of step b) and recovering crude lercanidipine hydrochloride Form (B)
a) reacting 2,6-dimethyl-5-methoxycarbonyl-4-(3-nitrophenyl)-1,4-dihydropyridine-3-carboxylic acid with a chloride selected from the group consisting of thionyl chloride and oxalyl chloride in an aprotic dipolar solvent and an aprotic polar solvent to produce the corresponding carbonyl chloride;
b) reacting, in-situ, the chloride of step a) with 2, N-dimethyl-N-(3,3-diphenylpropyl)-1-amino-2-propyl alcohol to yield crude lercanidipine hydrochloride; and c) isolating the crude lercanidipine hydrochloride of step b), washing the crude lercanidipine hydrochloride of step b) and recovering crude lercanidipine hydrochloride Form (B)
14. The method of claim 13 wherein the reacting step b) is conducted at a temperature between -5 and +5°C.
15. The method of claim 13 wherein step c) comprises the further steps of:
i') washing the crude lercanidipine hydrochloride of step b) with water, ii') removing the water from step i') to produce a mixture having a water content of about 2%, measured according to Karl Fischer;
iii') concentrating the mixture of step ii') and adding solvent to produce a solution having about the same volume as the initial volume of the mixture of step ii') and a water content, according to Karl Fischer, of between 0.9 and 1.1%;
iv') cooling the solution of step iii') to obtain a solid;
v') filtering the solid of step iv');
vi') re-suspending the solid of step v') in a solvent;
vii') cooling the suspension of step vi') to produce a solid; and viii') filtering and drying the solid at about 70°C to produce the crude lercanidipine hydrochloride Form (B).
i') washing the crude lercanidipine hydrochloride of step b) with water, ii') removing the water from step i') to produce a mixture having a water content of about 2%, measured according to Karl Fischer;
iii') concentrating the mixture of step ii') and adding solvent to produce a solution having about the same volume as the initial volume of the mixture of step ii') and a water content, according to Karl Fischer, of between 0.9 and 1.1%;
iv') cooling the solution of step iii') to obtain a solid;
v') filtering the solid of step iv');
vi') re-suspending the solid of step v') in a solvent;
vii') cooling the suspension of step vi') to produce a solid; and viii') filtering and drying the solid at about 70°C to produce the crude lercanidipine hydrochloride Form (B).
16. The method of claim 13 wherein the chloride is thionyl chloride.
17. The method of claim 15 wherein step c) ii') comprises removing the water from step i') by azeotropic reflux to produce said mixture.
18. The method of claim 15 wherein step c) iii') comprises concentrating said mixture to 3/4 of its initial volume.
19. The method of claim 15 wherein said solvent in steps c) iii') and vi') is ethyl acetate.
20. The method of claim 15 wherein the step c) iv') comprises cooling the solution to a temperature within the range of 0-5°C.
21. The method of claim 15 wherein said step c) vi') further comprises stirring the suspension at 60-65°C for about one hour.
22. The method of claim 21 wherein said step c) vii') further comprises cooling the solid to a temperature between 5 and 10°C.
23. The method of claim 15 wherein said drying in step viii') in an oven.
24. The method of any one of claims 1-7, wherein said aprotic dipolar solvent is dimethylformamide and said aprotic polar solvent is ethyl acetate.
25. Isolated lercanidipine hydrochloride crystalline Form (1), which has the X-ray diffraction pattern, at wavelength K , as shown in Figure 11.
26. The lercanidipine crystalline Form of claim 10, wherein distances, (I/Io) ratios, and 2 .theta. angles of significant peaks in Figure 11 are:
D (X) Relative intensity(I/Io)~2 .theta. angle 16.3 83 ~~5.4 6.2 47 ~~14.2 4.78 29 ~~18.6 4.10 63 ~~21.7 4.06 36 ~~21.9 3.90 100 ~~ 22.8
D (X) Relative intensity(I/Io)~2 .theta. angle 16.3 83 ~~5.4 6.2 47 ~~14.2 4.78 29 ~~18.6 4.10 63 ~~21.7 4.06 36 ~~21.9 3.90 100 ~~ 22.8
27. Isolated lercanidipine hydrochloride crystalline Form (II), which has an X-ray diffraction pattern, at wavelength K , as shown in Figure 12.
28. The lercanidipine crystalline Form of claim 27, wherein distances, (I/Io) ratios, and 2 .theta. angles of significant peaks in Figure 12 are:
D (X) Relative intensity(I/Io) ~2 .theta. angle 9.3 35 9.5 6.0 45 14.7 5.49 65 16.1 4.65 52 19.1 4.27 74 20.8 3.81 41 23.4 3.77 100 23.6 3.58 44 24.8 3.54 29 25.2
D (X) Relative intensity(I/Io) ~2 .theta. angle 9.3 35 9.5 6.0 45 14.7 5.49 65 16.1 4.65 52 19.1 4.27 74 20.8 3.81 41 23.4 3.77 100 23.6 3.58 44 24.8 3.54 29 25.2
29. A method of producing lercanidipine hydrochloride crystalline Form (I), which has an X-ray diffraction pattern, at wavelength K, as shown in Figure 11, which comprises:
d) adding isopropanol solvent to a crude lercanidipine hydrochloride Form and heating under reflux and with stirring to produce a clear solution;
e) cooling the solution of step d) and stirring until the concentration of lercanidipine hydrochloride dissolved in the crystallization solvent is #2%; and f) recovering the solid obtained from step e), and drying said solid to produce the lercanidipine hydrochloride crystalline Form (I).
d) adding isopropanol solvent to a crude lercanidipine hydrochloride Form and heating under reflux and with stirring to produce a clear solution;
e) cooling the solution of step d) and stirring until the concentration of lercanidipine hydrochloride dissolved in the crystallization solvent is #2%; and f) recovering the solid obtained from step e), and drying said solid to produce the lercanidipine hydrochloride crystalline Form (I).
30. The method of claim 29, wherein said step comprises filtering the solid obtained from step e) washing the solid with a C1-C5 alcohol containing a maximum 5% of water and re-filtering the solid before drying.
31. The method of claim 30 wherein the alcohol of step f) is selected from the group consisting of isopropanol, ethanol and anhydrous ethanol.
32. The method of claim 29, wherein the crude Form is lercanidipine hydrochloride crude Form (A) or lercanidipine hydrochloride crude Form (B).
33. The method of claim 29 wherein said step d) further comprises filtering the heated solution.
34. The method of claims 29 wherein said step e) comprises cooling the solution to a temperature between 30 and 40°C.
35. The method of claim 34 wherein said step e) further comprises stirring for a period of time of 12-48 hours.
36. The method of claim 29 wherein drying in said step f) takes place in an oven.
37. A method of producing lercanidipine hydrochloride crystalline Form (II), which has an x-ray diffraction pattern, at wavelength K.alpha., as shown in Figure 12, the method comprising the steps of:
d") adding acetonitrile to lercanidipine hydrochloride and heating the mixture thus obtained to form a solution;
e") cooling of the solution of step d") and stirring until the concentration of lercanidipine hydrochloride dissolved in the crystallization solvent is #2%; and f") filtering the solid of step a") and drying the solid in an oven to produce the lercanidipine hydrochloride Form (II).
d") adding acetonitrile to lercanidipine hydrochloride and heating the mixture thus obtained to form a solution;
e") cooling of the solution of step d") and stirring until the concentration of lercanidipine hydrochloride dissolved in the crystallization solvent is #2%; and f") filtering the solid of step a") and drying the solid in an oven to produce the lercanidipine hydrochloride Form (II).
38. The method of claim 37 wherein said step d") comprises heating said mixture under reflux with stirring.
39. The method of claim 37 wherein said step a") comprises cooling he solution to room temperature.
40. The method of claim 39 wherein said step a") comprises stirring the solution at room temperature for 24 hours.
41. The method of claim 37 Wherein drying step f") takes place in an oven.
42. The method of claim 37, wherein the crude Form is lercanidipine hydrochloride crude Form (A) or lercanidipine hydrochloride crude Form (B).
43. A method of producing lercanidipine hydrochloride crystalline Form (I), which has an x-ray diffraction pattern, at wavelength K.alpha., as shown in Figure 12, which comprises:
d') adding ethanol to lercanidipine hydrochloride, refluxing under stirring and cooling to form crystalline seeds of Form (I);
e') further cooling the seeded mixture of step d') and stiring until the concentration of lercanidipine hydrochloride dissolved in the crystallization solvent is #2%;
and ~) filtering the solid of step e') and drying said solid in an oven at 70°C to form lercanidipine hydrochloride Form (I).
d') adding ethanol to lercanidipine hydrochloride, refluxing under stirring and cooling to form crystalline seeds of Form (I);
e') further cooling the seeded mixture of step d') and stiring until the concentration of lercanidipine hydrochloride dissolved in the crystallization solvent is #2%;
and ~) filtering the solid of step e') and drying said solid in an oven at 70°C to form lercanidipine hydrochloride Form (I).
44. The method of claim 43 wherein the ratio of the weight of lercanidipine hydrochloride/ volume of solvent in step d') is within the range 1:4 to 1:6.
45. The method of claim 44 wherein said ratio is 1:4.
46. The method of claim 43 wherein said step d') further comprises filtering the heated solution.
47. The method of claim 43 wherein cooling in said step d') is to a temperature of 20°C while stiring.
48. The method of claim 43 wherein cooling in said step e') is to a temperature between 10 and 15°C.
49. The method of claim 43 wherein drying in said step f') takes place in oven, at 70°C.
50. The method of claim 47 wherein authentic seeds of lercanidipine Form I
are added at the end of cooling.
are added at the end of cooling.
51. A method of producing lercanidipine hydrochloride crystalline Form (II), which has an X-ray diffraction pattern, at wavelength K , as shown in Figure 12, which comprises:
d''') adding ethanol or isopropanol with a water content below 10% by weight to lercanidipine hydrochloride and refluxing to produce a solution;
e''') cooling the solution and stirring until the concentration of lercanidipine hydrochloride dissolved in the crystallization solvent is #2%; and f") filtering the solid and drying to produce lercanidipine hydrochloride Form (II).
d''') adding ethanol or isopropanol with a water content below 10% by weight to lercanidipine hydrochloride and refluxing to produce a solution;
e''') cooling the solution and stirring until the concentration of lercanidipine hydrochloride dissolved in the crystallization solvent is #2%; and f") filtering the solid and drying to produce lercanidipine hydrochloride Form (II).
52. The method of claim 51 wherein ethanol is added in said step d''')
53. The method of claims 51 wherein the water content in step d''') is between 10 and 5%.
54. The method of claim 51 wherein cooling in said step e''') is to a temperature between 20 and 40°C.
55. The method of claim 51 wherein drying in said step f''') takes place in an oven.
56. A method of producing the lercanidipine hydrochloride crystalline Form (II), which has an x-ray diffraction pattern, at wavelength K.alpha., as shown in Figure 12, which comprises:
d'''') dissolving crude lercanidipine hydrochloride or its crystalline Form (I) in protic polar or aprotic Bipolar solvents containing up to 50% by weight of water to produce a solution;
a"") stirring the solution of step d'''') until the concentration of lercanidipine hydrochloride dissolved in the crystallization solvent is #2%; and e'''') filtering and drying the solid of step e'''').
d'''') dissolving crude lercanidipine hydrochloride or its crystalline Form (I) in protic polar or aprotic Bipolar solvents containing up to 50% by weight of water to produce a solution;
a"") stirring the solution of step d'''') until the concentration of lercanidipine hydrochloride dissolved in the crystallization solvent is #2%; and e'''') filtering and drying the solid of step e'''').
57. The method of claim 56, further comprising irradiating with ultrasound and/or adding crystalline seeds of Form (II) to step e'''').
58. The method of claim 56, further comprising adding up to 60% water to the solution of step d'''').
59. The method of claim 56, wherein the protic polar solvent is an alcohol solvent
60. The method of claim 56, wherein the alcohol solvent is selected from the group consisting of methanol, ethanol, n-propanol, isopropanol.
61. The method of claim 56, wherein the aprotic dipolar solvent is N-methyl-pyrrolidone.
62. The method of claim 56, wherein the temperature of said step d'''') is between 20 and 70°C.
63. The method of claim 56, wherein stirring in said step e'''') takes place at a temperature between 20 and 25°C.
64. The method of claim 56, wherein drying in said step f'''') takes place at 70°C.
65. An antihypertensive pharmaceutical composition comprising (1) lercanidipine hydrochloride, wherein the lercanidipine hydrochloride is selected from the group consisting of lercanidipine hydrochloride crystalline Form (I), lercanidipine hydrochloride crystalline Form (II)and combinations thereof, of predetermined content in each of said Forms (I) and (II) and (2) at least one component selected from the group consisting of a pharmaceutically acceptable carrier or diluent, a flavorant, a sweetener, a preservative, a dye, a binder, a suspending agent, a dispersing agent, a colorant, a disintegrant, an excipient, a lubricant, a plasticizer, and an edible oil.
66. A unit dosage form comprising the antihypertensive pharmaceutical composition of claim 65.
67. The unit dosage form of claim 66, wherein the composition comprises 0.1 to 400 mg lercanidipine hydrochloride.
68. The unit dosage form of claim 67, wherein the composition comprises 1 to 200 mg lercanidipine hydrochloride.
69. The unit dosage form of claim 68, wherein the composition comprises 5 to 40 mg lercanidipine hydrochloride.
70. A method of treating a subject with arterial hypertension, the method comprising administering a therapeutically effective amount of lercanidipine hydrochloride crystalline Form (I), lercanidipine hydrochloride crystalline Form (II), or combinations hereof to a subject in need of such treatment.
71. A method of treating or preventing atherosclerotic lesions in arteries in a subject, which comprises administering a therapeutically effective amount of lercanidipine hydrochloride crystalline Form (I), lercanidipine hydrochloride crystalline Form (II), or combinations thereof having a predetermined content in each of said Form I and II to a subject in need of such treatment.
72. An antihypertensive composition comprising predetermined amounts of lercanidipine hydrochloride crystalline Form (I) and lercanidipine hydrochloride crystalline Form (II).
73. The antihypertensive composition of claim 72 wherein the lercanidipine hydrochloride crystalline Form (I) has a melting point of about 197-201 EC and the lercanidipine hydrochloride crystalline Form (II) has a melting point of about 207-211 EC, when said melting points are determined as DSC peaks.
74. The antihypertensive composition of claim 72 or claim 73 wherein the ratio of Form (I) : Form (II) is between 1:9 to 9:1.
75. The antihypertensive composition of claim 74 wherein the ratio of Form (I) : Form (II) is selected from the group consisting of 9:1, 7:3, 1:1, 3:7 and 1:9.
76. The isolated lercanidipine crystal Form of any one of claims 25, 26, 27 or 28 comprising an average particle size of D (50%) 2-8 µm and D (90%) < 15 µm.
77. The antihypertensive pharmaceutical composition of claim 65 wherein said lercanidipine hydrochloride crystalline Forms (I) and (II) each have an average particle size of D (50%) 2-8 µm and D (90%) < 15 µm.
78. The antihypertensive composition of any one of claims 72-75 wherein said lercanidipine crystalline Forms (I) and (II) each have an average particle size of D (50%) 2-8 µm and D (90%) < 15 µm.
Priority Applications (2)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CA2399459A CA2399459C (en) | 2001-08-06 | 2002-08-06 | Novel crude and crystalline forms of lercanidipine hydrochloride |
| CA 2399583 CA2399583A1 (en) | 2001-08-06 | 2002-08-06 | Novel solvate and crystalline forms of lercanidipine hydrochloride |
Applications Claiming Priority (4)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| IT2001MI001726A ITMI20011726A1 (en) | 2001-08-06 | 2001-08-06 | POLYMORPHIC FORMS OF LERCANIDIPINE HYDROCHLORIDE |
| ITM12001A011726 | 2001-08-06 | ||
| US36778902P | 2002-03-26 | 2002-03-26 | |
| US60/367,789 | 2002-03-26 |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| CA2380202A1 true CA2380202A1 (en) | 2003-02-06 |
Family
ID=26332786
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA 2380202 Abandoned CA2380202A1 (en) | 2001-08-06 | 2002-04-03 | Novel crude and crystalline forms of lercanidipine hydrochloride |
Country Status (1)
| Country | Link |
|---|---|
| CA (1) | CA2380202A1 (en) |
-
2002
- 2002-04-03 CA CA 2380202 patent/CA2380202A1/en not_active Abandoned
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