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JPH0840908A - Cancerous cell proliferation inhibitor - Google Patents

Cancerous cell proliferation inhibitor

Info

Publication number
JPH0840908A
JPH0840908A JP17661994A JP17661994A JPH0840908A JP H0840908 A JPH0840908 A JP H0840908A JP 17661994 A JP17661994 A JP 17661994A JP 17661994 A JP17661994 A JP 17661994A JP H0840908 A JPH0840908 A JP H0840908A
Authority
JP
Japan
Prior art keywords
cancer
membered
compound
active ingredient
cck
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.)
Pending
Application number
JP17661994A
Other languages
Japanese (ja)
Inventor
Kazuo Chihara
和夫 千原
Toshimitsu Matsui
利充 松井
Mitsuhiro Ito
光宏 伊藤
Taizo Taniguchi
泰造 谷口
Noboru Iwata
暢 岩田
Toru Murayama
徹 村山
Masato Sato
正人 佐藤
Current Assignee (The listed assignees may be inaccurate. Google has not performed a legal analysis and makes no representation or warranty as to the accuracy of the list.)
Yamanouchi Pharmaceutical Co Ltd
Original Assignee
Yamanouchi Pharmaceutical Co Ltd
Priority date (The priority date 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 date listed.)
Filing date
Publication date
Application filed by Yamanouchi Pharmaceutical Co Ltd filed Critical Yamanouchi Pharmaceutical Co Ltd
Priority to JP17661994A priority Critical patent/JPH0840908A/en
Publication of JPH0840908A publication Critical patent/JPH0840908A/en
Pending legal-status Critical Current

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Abstract

PURPOSE:To obtain a cancerous cell proliferation inhibltor or medicine for cancer presenting medicinal virtues to inhibit ligand-dependent cell proliferation such as for CCK-8 or gastrin, containing, as active ingredient, a specific benzodiazepine derivative or a pharmaceutically permissible salt thereof. CONSTITUTION:This cancerous cell proliferation inhibitor or medicine for cancer contains, as active ingredient, a benzodiazepine derivative of the formula (R<1> is an aryl, five-membered monocyclc, six-membered monocyclic or five- membered-six-membered condensed aromatic heterocyclic group; R<2> is an aryl) or a pharmaceutically permissible salt thereof. The compound of the formula is esp. (R)-1-[2,3-dihydro-1-(2'-methylphenacyl)-2-oxo-5-phenyl-1H-1,4- benzodiazepin-3-yl]-3-(3-tolyl) urea or a pharmaceutically permissible salt thereof. This active ingredient, which inhibit rapid proliferation to be termed a characteristic of cancerous cell, is useful as a medicine for pulmonary cancer, pancreatic cancer, colon cancer, gastric cancer, T-cell lymphoma, etc., being also useful as a cancer diagnostic.

Description

【発明の詳細な説明】Detailed Description of the Invention

【0001】[0001]

【産業上の利用分野】本発明は、医薬として有用な、殊
に一般式FIELD OF THE INVENTION The present invention relates to a compound of general formula

【化2】 (式中の記号は、以下の意味を示す。 R1:置換されていてもよいアリール基又は5員単環、
6員単環もしくは5員−6員連環の芳香族複素環基。 R2:置換されていてもよいアリール基。)で示される
ベンゾジアゼピン誘導体又はその製薬学的に許容される
塩を有効成分とする癌細胞増殖抑制剤並びに癌治療薬に
関する。Embedded image (The symbols in the formulas have the following meanings: R 1 : an optionally substituted aryl group or a 5-membered monocycle,
A 6-membered monocyclic or 5-membered to 6-membered continuous aromatic heterocyclic group. R 2: an aryl group which may be substituted. ), A benzodiazepine derivative or a pharmaceutically acceptable salt thereof as an active ingredient, and a cancer cell growth inhibitor and a cancer therapeutic agent.

【0002】[0002]

【従来の技術・発明が解決しようとする課題】本発明医
薬の有効成分である一般式(I)で示される化合物又は
その塩は、CCK−B(コレシストキニン−Brai
n)受容体及びガストリン受容体拮抗作用を有すること
から、胃潰瘍、十二指腸潰瘍、胃炎等の消化器系疾患や
食欲調整系の障害、痛み、不安等の中枢系の障害等に有
用なことが知られている(国際公開第92/11246
号パンフレット(1992))。ヒト大脳CCK−B受
容体とガストリン受容体は、遺伝子クローニングにより
同一であることが示され(J.Biol.Chem.268,18300(199
3),J.Biol.Chem.268,8164(1993))、肺癌、膵癌、大腸
癌、胃癌、T細胞性リンパ腫等の多くのヒト癌細胞株に
発現している。これらヒト癌細胞株は、CCKやガスト
リン等のリガンドによって濃度依存的に増殖することが
知られている(Am.J.Physiol.266,277(1994),Cancer Re
s.53,5208(1993),Cancer Res.49,2840(1989),Oncogene
9,861(1994))。一方、選択的なCCK−B/ガストリ
ン受容体拮抗薬であるL−365260(米国特許第
4,820,834号明細書 実施例281記載の化合
物)は、ヒト肺小細胞癌由来の細胞株において,CCK
の生物活性を示す部分ペプチドであるCCK−8の特異
的結合を阻害することが報告されているが(Peptides
8,103(1987),Peptides 11,1033(1990))、この化合物の
CCK−B/ガストリン受容体に対する結合阻害活性は
弱く、臨床において癌治療薬として応用されるまでには
至っていない。2. Description of the Related Art The compound represented by the general formula (I) or a salt thereof, which is an active ingredient of the medicament of the present invention, is CCK-B (cholecystokinin-Brai).
n) Receptor and gastrin receptor antagonistic action is known to be useful for digestive system diseases such as gastric ulcer, duodenal ulcer, gastritis and disorders of central nervous system such as appetite regulation system, pain and anxiety. (International Publication No. 92/11246
Issue pamphlet (1992)). Human cerebral CCK-B receptor and gastrin receptor have been shown to be identical by gene cloning (J. Biol. Chem. 268 , 18300 (199).
3), J. Biol. Chem. 268 , 8164 (1993)), lung cancer, pancreatic cancer, colon cancer, gastric cancer, T-cell lymphoma, and many other human cancer cell lines. These human cancer cell lines, are known to grow a concentration-dependent manner by a ligand such as CCK or gastrin (Am.J.Physiol. 266, 277 (1994 ), Cancer Re
s. 53 , 5208 (1993), Cancer Res. 49 , 2840 (1989), Oncogene
9 , 861 (1994)). On the other hand, L-365260 (a compound described in US Pat. No. 4,820,834, Example 281), which is a selective CCK-B / gastrin receptor antagonist, was used in a cell line derived from human small cell lung cancer. , CCK
Has been reported to inhibit the specific binding of CCK-8, which is a partial peptide showing biological activity of Peptides (Peptides
8 , 103 (1987), Peptides 11 , 1033 (1990)), the binding inhibitory activity of this compound on the CCK-B / gastrin receptor is weak, and it has not been clinically applied as a therapeutic drug for cancer.

【0003】[0003]

【課題を解決するための手段】本発明者等は、CCK−
B/ガストリン受容体拮抗作用を有する上記一般式
(I)で示される化合物について鋭意研究を行った結
果、これらの化合物がCCK−8やガストリン等のリガ
ンド依存性の細胞増殖を抑制することを見い出し、本発
明を完成した。即ち、本発明は、一般式(I)で示され
る化合物又はその塩を有効成分とするCCK−B/ガス
トリン受容体発現癌細胞の増殖抑制剤に関する。殊に、
本発明は癌細胞に発現したCCK−B/ガストリン受容
体に結合し、CCK及びガストリンの作用に拮抗する化
合物を含有する医薬を提供することを目的とする。更
に、本発明の有効成分である一般式(I)で示される化
合物は、CCK−B/ガストリン受容体を発現する癌細
胞内のDNA合成をも抑制して、癌細胞増殖抑制作用を
示す。The present inventors have found that the CCK-
As a result of intensive studies on compounds represented by the above general formula (I) having B / gastrin receptor antagonistic action, they found that these compounds suppress ligand-dependent cell growth of CCK-8, gastrin and the like. The present invention has been completed. That is, the present invention relates to a CCK-B / gastrin receptor-expressing cancer cell growth inhibitor containing a compound represented by the general formula (I) or a salt thereof as an active ingredient. In particular,
An object of the present invention is to provide a drug containing a compound that binds to CCK-B / gastrin receptor expressed in cancer cells and antagonizes the actions of CCK and gastrin. Furthermore, the compound represented by the general formula (I), which is an active ingredient of the present invention, also suppresses DNA synthesis in cancer cells expressing CCK-B / gastrin receptor and exhibits a cancer cell growth inhibitory action.

【0004】ここに一般式(I)で示される化合物にお
いて「アリール基」としては、たとえばフェニル基、イ
ンデニル基及びナフチル基等が挙げられる。これらのア
リール基は置換基を有していてもよい。この置換基とし
てはたとえば、低級アルキル基、低級アルコキシ基及び
ハロゲン原子等を挙げることができる。ここに、低級ア
ルキル基とは、炭素数1〜6個からなる直鎖上又は分枝
状の炭化水素鎖であり、代表的なものとしては、メチル
基、エチル基、プロピル基,n−ブチル基,n−ペンチ
ル基、イソプロピル基、sec−ブチル基等である。ま
た、低級アルコキシ基とは、上記低級アルキル基を有す
るアルコキシ基であって、たとえばメトキシ基、エトキ
シ基、プロポキシ基、イソプロポキシ基、n−ブトキシ
基等を挙げることができる。ハロゲン原子としては、た
とえばフッ素原子、塩素原子又は臭素原子が挙げられ
る。次に、「5員単環、6員単環もしくは5員−6員連
環の芳香族複素環基」としてはチオフェン環、フラン
環、ピロール環、チアゾール環、オキサゾール環、イミ
ダゾール環、ピリジン環、ベンゾチオフェン環、ベンゾ
フラン環、インドール環等を挙げることができる。Examples of the "aryl group" in the compound represented by formula (I) include a phenyl group, an indenyl group and a naphthyl group. These aryl groups may have a substituent. Examples of this substituent include a lower alkyl group, a lower alkoxy group and a halogen atom. Here, the lower alkyl group is a linear or branched hydrocarbon chain having 1 to 6 carbon atoms, and typical examples thereof include a methyl group, an ethyl group, a propyl group, and n-butyl. Group, n-pentyl group, isopropyl group, sec-butyl group and the like. The lower alkoxy group is an alkoxy group having the above lower alkyl group, and examples thereof include a methoxy group, an ethoxy group, a propoxy group, an isopropoxy group, and an n-butoxy group. Examples of the halogen atom include a fluorine atom, a chlorine atom or a bromine atom. Next, as the "5-membered monocyclic, 6-membered monocyclic or 5-membered-6-membered aromatic heterocyclic group", a thiophene ring, a furan ring, a pyrrole ring, a thiazole ring, an oxazole ring, an imidazole ring, a pyridine ring, Examples thereof include a benzothiophene ring, a benzofuran ring and an indole ring.

【0005】次に、本発明の有効成分である化合物
(I)は、不整炭素原子を有しており、異性体が存在す
るため、本発明の有効成分として、これらの異性体をも
採用することができる。また、本発明化合物は、酸と塩
を形成する。それらの塩としては、たとえば塩酸塩、硫
酸塩、酢酸塩等の無機酸又は有機酸との塩が挙げられ
る。尚、化合物(I)及びその塩の製造法については、
国際公開第92/11246号パンフレット(199
2)に係る出願に記載されている。Next, since the compound (I), which is the active ingredient of the present invention, has an asymmetric carbon atom and has isomers, these isomers are also adopted as the active ingredient of the present invention. be able to. Further, the compound of the present invention forms a salt with an acid. Examples of such salts include salts with inorganic acids or organic acids such as hydrochlorides, sulfates and acetates. In addition, about the manufacturing method of compound (I) and its salt,
International Publication No. 92/11246 Pamphlet (199
It is described in the application pertaining to 2).

【0006】[0006]

【発明の効果】本発明医薬の有効成分である一般式
(I)で示される化合物又はその塩は、癌細胞の特質と
もいえる急速な増殖を抑制するため、肺癌、膵癌、大腸
癌、胃癌、T細胞性リンパ腫等の癌治療薬として有用で
ある。更には、癌細胞に発現したCCK−B/ガストリ
ン受容体へのリガンド結合阻害作用により、癌細胞のC
CK及びガストリンに対する感受性を検出することも可
能であり、癌診断薬としても有用である。INDUSTRIAL APPLICABILITY The compound represented by the general formula (I) or a salt thereof, which is an active ingredient of the medicament of the present invention, suppresses rapid proliferation, which can be said to be characteristic of cancer cells, and therefore lung cancer, pancreatic cancer, colon cancer, gastric cancer It is useful as a therapeutic drug for cancer such as T cell lymphoma. Furthermore, the CCK-B of the cancer cells / the gastrin receptor is inhibited by the ligand binding inhibitory action to the C of the cancer cells.
It is also possible to detect sensitivity to CK and gastrin, and it is also useful as a cancer diagnostic agent.

【0007】また、本発明の化合物は毒性が低く、医薬
としての使用に適している。たとえばSDラットの試験
では、経口投与において100mg/kg投与しても重
篤な副作用は認められない。本発明化合物又はその塩は
錠剤、散剤、細粒剤、カプセル剤、丸剤、液剤、注射
剤、坐剤、軟膏、貼付剤等に調整され、経口的(舌下投
与を含む)又は非経口的に投与される。製剤用の単体や
賦形剤としては、個体又は液体状の非毒性医薬用物質が
挙げられる。これらの例としては、たとえば乳糖、ステ
アリン酸マグネシウム、スターチ、タルク、ゼラチン、
寒天、ペクチン、アラビアゴム、オリーブ油、ゴマ油、
カカオバター、エチレングリコール等やその他常用のも
のが例示される。本発明化合物の臨床的投与量は、適用
される患者の症状、体重、年齢や性別等を考慮して適宜
決定されるが、通常成人1日あたり経口投与で1〜10
00mgであり、これを1回あるいは数回に分けて投与
する。The compound of the present invention has low toxicity and is suitable for use as a medicine. For example, in the SD rat test, no serious side effect was observed even when 100 mg / kg was orally administered. The compound of the present invention or a salt thereof is adjusted to tablets, powders, fine granules, capsules, pills, solutions, injections, suppositories, ointments, patches and the like, and is orally (including sublingual administration) or parenteral. Will be given to you. Examples of the simple substance or excipient for the preparation include solid or liquid non-toxic medicinal substances. Examples of these are lactose, magnesium stearate, starch, talc, gelatin,
Agar, pectin, gum arabic, olive oil, sesame oil,
Examples include cocoa butter, ethylene glycol, and other commonly used ones. The clinical dose of the compound of the present invention is appropriately determined in consideration of the symptoms, weight, age, sex, etc. of the patient to whom it is applied, but it is usually 1 to 10 by oral administration per day for an adult.
The dose is 00 mg, which is to be administered once or in several divided doses.

【0008】〈実験例及び実施例〉次に、実験例及び実
施例を挙げて、本発明を更に説明する。 実験例1(ヒト癌細胞の増殖抑制作用) 実験系の意義 DNAの前駆体であるチミジンの細胞への取り込み量を
測定することにより,DNA合成を指標に細胞増殖抑制
作用を測定した。下記実験例及び実施例においては、被
験化合物として一般式(I)で示される化合物のうち
(R)−1−[2,3−ジヒドロ−1−(2’−メチル
フェナシル)−2−オキソ−5−フェニル−1H−1,
4−ベンゾジアゼピン−3−イル]−3−(3−トリ
ル)ウレア(以下、化合物Aと称する)を、その対照化
合物としてL−365260(米国特許第4,820,
834号明細書 実施例281に記載の化合物)を採用
した。<Experimental Examples and Examples> The present invention will be further described with reference to Experimental Examples and Examples. Experimental Example 1 (Human Cancer Cell Proliferation Inhibitory Action) Significance of Experimental System The cell proliferation inhibitory action was measured using DNA synthesis as an index by measuring the uptake of thymidine, which is a precursor of DNA, into cells. In the following Experimental Examples and Examples, (R) -1- [2,3-dihydro-1- (2′-methylphenacyl) -2-oxo among the compounds represented by the general formula (I) was used as a test compound. -5-phenyl-1H-1,
4-Benzodiazepin-3-yl] -3- (3-tolyl) urea (hereinafter referred to as Compound A) was used as a control compound thereof in L-365260 (US Pat. No. 4,820,
No. 834, the compound described in Example 281) was adopted.

【0009】実験方法 ヒト肺小細胞癌由来のNCIH510A細胞を、10%
牛胎児血清を添加したRPMI1640培地(Gibuco社
Grand Island,NY)中で37℃、5%CO2下で培養維
持したものを使用した。血清飢餓にした上記細胞を96
穴プレートに播種し、インスリン、トランスフェリン添
加RPMI培地中にガストリン(10-8M)及び各種濃
度の被験化合物又は対照化合物を添加して44時間培養
を行い、続いてメチル[3H]チミジン(1Ciml、25mCi/m
mol,Amersham)を添加して4時間培養を行った。培養
後、トリクロロ酢酸(5%)を加えて、遠心分離により
取り込まれなかったチミジンを除去し、沈殿(細胞)を
1%SDS添加1mM水酸化ナトリウムで溶解した。液
体シンチレーションカウンターで[3H]量を測定し
て、細胞内に取り込まれたチミジン量とした。この結果
を図1に示す。本結果より、被験化合物は10-7M以上
でDNA合成におけるチミジン取り込みを抑制したこと
から、癌細胞増殖を有意に抑制することが判明した。一
方、対照化合物であるL−365260は被験化合物の
10倍量で同等程度のチミジン取り込みを抑制したこと
から、癌細胞増殖抑制効果において、本発明化合物は、
対照化合物の10倍以上の効果を有することが分った。Experimental Method NCIH510A cells derived from human small cell lung cancer were 10%
RPMI 1640 medium supplemented with fetal bovine serum (Gibuco
Cultured and maintained in Grand Island, NY) at 37 ° C. under 5% CO 2 was used. 96 cells above serum-starved
Seed on a well plate, add gastrin (10 -8 M) and various concentrations of test compound or control compound to RPMI medium supplemented with insulin and transferrin, and incubate for 44 hours, followed by methyl [ 3 H] thymidine (1 Ciml , 25mCi / m
mol, Amersham) was added and the cells were cultured for 4 hours. After culturing, trichloroacetic acid (5%) was added to remove thymidine that was not incorporated by centrifugation, and the precipitate (cells) was lysed with 1 mM SDS-added 1 mM sodium hydroxide. The amount of [ 3 H] was measured with a liquid scintillation counter and used as the amount of thymidine incorporated into cells. The result is shown in FIG. From this result, it was revealed that the test compound significantly inhibited the growth of cancer cells because it inhibited thymidine incorporation in DNA synthesis at 10 −7 M or more. On the other hand, the control compound L-365260 suppressed the thymidine uptake to the same extent with a 10-fold amount of the test compound.
It was found to be 10 times more effective than the control compound.

【0010】実験例2(ヒトCCK−B/ガストリン受
容体発現マウス細胞の増殖抑制作用) 実験系の意義 CCK及びガストリンの細胞増殖促進作用は、CCK又
はガストリンが細胞表面に存在するCCK−B/ガスト
リン受容体に結合することにより、イノシトールリン酸
や細胞内Ca2+等を介する細胞内情報伝達機構が活性化
され、その増幅したシグナルが核に到達し、核内のDN
A合成が促進されることにより、細胞増殖に到ると考え
られている。そこで、ヒトのCCK−B/ガストリン受
容体を発現させたマウスの繊維芽細胞(非癌細胞)を用
い、細胞内情報伝達因子であるイノシトールリン酸産生
を指標に、本発明化合物によるCCKのCCK−B/ガ
ストリン受容体発現細胞への結合阻害、及びそれに伴う
細胞内情報伝達機構の活性化抑制と細胞増殖抑制効果を
確認した。ここで、以下の実験で用いたCCK−8は、
CCKの部分ペプチドであり26〜33までの8アミノ
酸残基を有し、CCK−B/ガストリン受容体のリガン
ド作用を示す(Yalow:Gastroenterology.58,609(197
0))。Experimental Example 2 (Inhibition of proliferation of human CCK-B / gastrin receptor-expressing mouse cells) Significance of the experimental system The cell proliferation promoting action of CCK and gastrin is CCK-B / in which CCK or gastrin is present on the cell surface. By binding to the gastrin receptor, the intracellular signal transduction mechanism via inositol phosphate, intracellular Ca 2+, etc. is activated, and the amplified signal reaches the nucleus and DN in the nucleus is activated.
It is believed that the promotion of A synthesis leads to cell proliferation. Therefore, using mouse fibroblasts (non-cancerous cells) expressing human CCK-B / gastrin receptor, CCK of CCK by the compound of the present invention is used with the production of inositol phosphate, which is an intracellular signal transduction factor, as an index. -Inhibition of binding to B / gastrin receptor-expressing cells, and accompanying suppression of activation of intracellular signal transduction mechanism and suppression of cell proliferation were confirmed. Here, CCK-8 used in the following experiments is
It is a partial peptide of CCK and has 8 amino acid residues from 26 to 33, and exhibits a ligand action of CCK-B / gastrin receptor (Yalow: Gastroenterology. 58 , 609 (197
0)).

【0011】実験方法 ヒトCCK−B/ガストリン受容体を発現したマウス繊
維芽細胞株NIH3T3細胞(Taniguchi et al.:Oncog
ene 9,861(1994))を10%牛血清(ICN Flow,Costa Me
sa、CA)を添加したDMEM培地(Gibuco、Grand Islan
d、NY)中で培養維持したものを使用した。血清飢餓にし
た上記細胞をmyo[3H]イノシトール(1μCiml、10
-20mCi/mmol,Amersham)で予め24時間標識を行った。
細胞をDMEM培地にて2回洗浄した後CCK−8(5
×10-9M)及び各種濃度の被験化合物又は対照化合物
を添加し、10mMクロロリチウム存在下37℃で30
分反応を行った。氷冷したメタノールの添加により反応
停止、イノシトールリン酸を抽出して、[3H]量を液
体シンチレーションカウンターにて測定し、イノシトー
ルリン酸産生量を求めた。この結果を図2に示す。本結
果より、本発明医薬の有効成分である一般式(I)で示
される化合物は、対照化合物に比して有意に強いイノシ
トールリン酸産生抑制効果を示した。即ち、化合物Aは
10-8M量で90%以上の抑制を示したのに対し、対照
化合物では抑制効果は見られなかった。これにより本発
明医薬の有効成分である化合物(I)はヒトCCK−B
/ガストリン受容体発現細胞において顕著な細胞内情報
伝達機構の活性化抑制を示したことから、細胞増殖抑制
効果がCCK−B/ガストリン受容体発現細胞への結合
阻害、及びそれに伴う細胞内情報伝達機構の活性化抑制
によるものであることを確認した。Experimental Method Mouse CHI-B / gastrin receptor-expressing mouse fibroblast cell line NIH3T3 cells (Taniguchi et al .: Oncog
ene 9, 861 (1994)) 10% bovine serum (ICN Flow, Costa Me
sa, CA) added DMEM medium (Gibuco, Grand Islan
d, NY) were used after being maintained in culture. The serum-starved cells were treated with myo [ 3 H] inositol (1 μCiml, 10
-20 mCi / mmol, Amersham) was preliminarily labeled for 24 hours.
After washing the cells twice with DMEM medium, CCK-8 (5
X 10 -9 M) and various concentrations of the test compound or control compound were added, and the mixture was incubated at 37 ° C in the presence of 10 mM chlorolithium for 30 minutes.
A minute reaction was performed. The reaction was stopped by the addition of ice-cooled methanol, inositol phosphate was extracted, and the [ 3 H] amount was measured by a liquid scintillation counter to determine the amount of inositol phosphate produced. The result is shown in FIG. From these results, the compound represented by the general formula (I), which is the active ingredient of the pharmaceutical composition of the present invention, showed a significantly stronger inositol phosphate production inhibitory effect than the control compound. That is, the compound A showed 90% or more inhibition at the amount of 10 -8 M, whereas the control compound did not show the inhibition effect. As a result, the compound (I), which is the active ingredient of the pharmaceutical composition of the present invention, was identified as human CCK-B
/ Gastrin receptor-expressing cells showed remarkable inhibition of activation of intracellular signal transduction mechanism. Therefore, the cell growth inhibitory effect is inhibition of binding to CCK-B / gastrin receptor-expressing cells and accompanying intracellular signal transduction. It was confirmed that it was due to suppression of activation of the mechanism.

【0012】[0012]

【実施例】以下に本発明の医薬について実施例により更
に詳細に説明する。 実施例1 (錠剤) 組 成 20mg錠 40mg錠 化合物A 20mg 40mg 乳糖 73.4 80 コーンスターチ 18 20 ヒドロキシプロピルセルロース 4 5 カルボキシメチルセルロースカルシウム 4 4.2 ステアリン酸マグネシウム 0.6 0.8 合 計 120mg 150mg EXAMPLES The medicine of the present invention will be described in more detail below with reference to examples. Example 1 (tablet) composition 20 mg tablet 40 mg tablet compound A 20 mg 40 mg lactose 73.4 80 corn starch 18 20 hydroxypropylcellulose 45 carboxymethylcellulose calcium 4 4.2 magnesium stearate 0.6 0.8 total 120 mg 150 mg

【0013】20mg錠の調整法 化合物A 100g、乳糖 367g,コーンスターチ
90gを流動造粒コーティング装置(大川原製作所
製)を使用して均一に混合した。これに10%ヒドロキ
シプロピルセルロース溶液 200gを噴霧して造粒し
た。乾燥後、20メッシュの篩を通し、これにカルボキ
シメチルセルロースカルシウム 20g、ステアリン酸
マグネシウム 3gを加え、ロータリー打錠機(畑鉄工
所製)で7mm×8.4Rの臼杵を使用して1錠当たり
120mgの錠剤とした。 Preparation Method of 20 mg Tablet Compound A (100 g), lactose (367 g) and corn starch (90 g) were uniformly mixed using a fluidized granulation coating apparatus (manufactured by Okawara Seisakusho). 200 g of a 10% hydroxypropyl cellulose solution was sprayed on this and granulated. After drying, it is passed through a 20-mesh sieve, 20 g of carboxymethylcellulose calcium and 3 g of magnesium stearate are added, and 120 mg per tablet is obtained using a rotary tableting machine (manufactured by Hata Tekko Co., Ltd.) with a 7 mm x 8.4 R pestle. As tablets.

【0014】40mg錠の調整法 化合物A 140g、乳糖 280g,コーンスターチ
70gを流動造粒コーティング装置(大川原製作所
製)を使用して均一に混合した。これに10%ヒドロキ
シプロピルセルロース溶液 175gを噴霧して造粒し
た。乾燥後、20メッシュの篩を通し、これにカルボキ
シメチルセルロースカルシウム 14.7g、ステアリ
ン酸マグネシウム 2.8gを加え、ロータリー打錠機
(畑鉄工所製)で7.5mm×9Rの臼杵を使用して1
錠当たり150mgの錠剤とした。 Preparation Method of 40 mg Tablet Compound A (140 g), lactose (280 g) and corn starch (70 g) were uniformly mixed using a fluidized granulation coating apparatus (manufactured by Okawara Seisakusho). 175 g of a 10% hydroxypropyl cellulose solution was sprayed on this and granulated. After drying, it was passed through a 20-mesh sieve, 14.7 g of carboxymethylcellulose calcium and 2.8 g of magnesium stearate were added thereto, and a rotary tableting machine (manufactured by Hata Tekko Co., Ltd.) was used to use a 7.5 mm × 9R pestle. 1
Each tablet was 150 mg.

【図面の簡単な説明】[Brief description of drawings]

【図1】化合物A及び対照化合物について、チミジンの
細胞内への取り込み量を比較した図である。FIG. 1 is a diagram comparing the amount of thymidine incorporated into cells for Compound A and a control compound.

【図2】化合物A及び対照化合物について、イノシトー
ルリン酸の産生量を比較した図である。FIG. 2 is a diagram comparing the amount of inositol phosphate produced for compound A and a control compound.

───────────────────────────────────────────────────── フロントページの続き (72)発明者 谷口 泰造 兵庫県神戸市北区日の峰5丁目10−1− 801 (72)発明者 岩田 暢 兵庫県神戸市東灘区住吉台14番8−208号 (72)発明者 村山 徹 兵庫県神戸市中央区多聞通5丁目2−7− 302号 (72)発明者 佐藤 正人 茨城県つくば市二の宮2丁目5番地の9 ルーミー筑波321号 ─────────────────────────────────────────────────── ─── Continuation of the front page (72) Taizo Taniguchi 5-10-1-801 Hinomine, Kita-ku, Kobe-shi, Hyogo (72) Inventor Nobu Akira Iwata 14-8-208 Sumiyoshidai, Higashinada-ku, Kobe-shi, Hyogo ( 72) Inventor Toru Murayama 5-2-7-302 Tamon-dori, Chuo-ku, Kobe-shi, Hyogo Prefecture (72) Masato Sato 9 Rumi Tsukuba 321 9-5 2-chome Ninomiya, Tsukuba, Ibaraki

Claims (3)

【特許請求の範囲】[Claims] 【請求項1】 一般式 【化1】 (式中の記号は、以下の意味を示す。 R1:置換されていてもよいアリール基又は5員単環、
6員単環もしくは5員−6員連環の芳香族複素環基。 R2:置換されていてもよいアリール基。)で示される
ベンゾジアゼピン誘導体又はその製薬学的に許容される
塩を有効成分とする癌細胞増殖抑制剤。1. A compound of the general formula (The symbols in the formulas have the following meanings: R 1 : an optionally substituted aryl group or a 5-membered monocycle,
A 6-membered monocyclic or 5-membered to 6-membered continuous aromatic heterocyclic group. R 2: an aryl group which may be substituted. ) A cancer cell growth inhibitor comprising a benzodiazepine derivative or a pharmaceutically acceptable salt thereof as an active ingredient. 【請求項2】 (R)−1−[2,3−ジヒドロ−1−
(2’−メチルフェナシル)−2−オキソ−5−フェニ
ル−1H−1,4−ベンゾジアゼピン−3−イル]−3
−(3−トリル)ウレア又はその製薬学的に許容される
塩を有効成分とする請求項1記載の癌細胞増殖抑制剤。2. (R) -1- [2,3-dihydro-1-
(2'-Methylphenacyl) -2-oxo-5-phenyl-1H-1,4-benzodiazepin-3-yl] -3
The cancer cell proliferation inhibitor according to claim 1, which comprises-(3-tolyl) urea or a pharmaceutically acceptable salt thereof as an active ingredient. 【請求項3】癌治療薬として用いる請求項1又は2記載
の癌細胞増殖抑制剤。3. The cancer cell growth inhibitor according to claim 1, which is used as a therapeutic drug for cancer.
JP17661994A 1994-07-28 1994-07-28 Cancerous cell proliferation inhibitor Pending JPH0840908A (en)

Priority Applications (1)

Application Number Priority Date Filing Date Title
JP17661994A JPH0840908A (en) 1994-07-28 1994-07-28 Cancerous cell proliferation inhibitor

Applications Claiming Priority (1)

Application Number Priority Date Filing Date Title
JP17661994A JPH0840908A (en) 1994-07-28 1994-07-28 Cancerous cell proliferation inhibitor

Publications (1)

Publication Number Publication Date
JPH0840908A true JPH0840908A (en) 1996-02-13

Family

ID=16016748

Family Applications (1)

Application Number Title Priority Date Filing Date
JP17661994A Pending JPH0840908A (en) 1994-07-28 1994-07-28 Cancerous cell proliferation inhibitor

Country Status (1)

Country Link
JP (1) JPH0840908A (en)

Cited By (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
WO1998002419A1 (en) * 1996-07-12 1998-01-22 Chugai Seiyaku Kabushiki Kaisha Cancer cell proliferation inhibitors
WO2002092096A1 (en) * 2001-05-11 2002-11-21 Yamanouchi Pharmaceutical Co., Ltd. Antitumor agents
WO2006077793A1 (en) * 2005-01-19 2006-07-27 Zeria Pharmaceutical Co., Ltd. Antitumor agent
CN113956246A (en) * 2021-10-25 2022-01-21 中山大学 2-phenyl-4H-benzo [1,3] oxazine derivative containing 3-phenyl furan and preparation and application thereof

Cited By (6)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
WO1998002419A1 (en) * 1996-07-12 1998-01-22 Chugai Seiyaku Kabushiki Kaisha Cancer cell proliferation inhibitors
WO2002092096A1 (en) * 2001-05-11 2002-11-21 Yamanouchi Pharmaceutical Co., Ltd. Antitumor agents
WO2006077793A1 (en) * 2005-01-19 2006-07-27 Zeria Pharmaceutical Co., Ltd. Antitumor agent
JP4957250B2 (en) * 2005-01-19 2012-06-20 ゼリア新薬工業株式会社 Antitumor agent
CN113956246A (en) * 2021-10-25 2022-01-21 中山大学 2-phenyl-4H-benzo [1,3] oxazine derivative containing 3-phenyl furan and preparation and application thereof
CN113956246B (en) * 2021-10-25 2023-09-22 中山大学 3-phenyl furan-containing 2-phenyl-4H-benzo [1,3] oxazine derivative and preparation and application thereof

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