DE3032072C2 - Method for the analysis of protein subunits with the aid of electrophoresis on thin layers which contain tetramethylurea or similar urea derivatives - Google Patents

Description

The invention relates to a method for analyzing protein subunits according to the generic term of the claim.

The electrophoresis of proteins, i.e. their separation due to different mobility behavior in an electrical direct voltage field, has the field of biochemistry and medical diagnostics has gained great importance. A specialty here consists in the separation of the subunits of proteins, which arise from the fact that one puts the proteins in a 50% urea solution. B. in four Subunits, the electrophoretic analysis of which is much clearer diagnostically for pathological changes The analysis of the whole hemoglobins (Altland, K. and Kämper, M. (1979) Human Genetics 53.97-100).

If this separation is carried out on freshly prepared layers of agarose or polyacrylamide in the laboratory, this must be carried out accordingly Contain an admixture of urea so that the subunits do not come together again naturally and complicate the separation process. If one wants to keep such electrophoretic layers ready for a long time and produce in an acceptable trade and shipping forms, it follows that finished layers containing such high concentrations of urea, have serious disadvantages.

1. Urea breaks down according to the following equation

H ₂ N- CO — NH ₂ «-» CNCr + NH ₄ ⁺ (1)

in ammonium cyanate.

The free cyanate reacts very quickly with the free amino groups contained in the proteins in the following way, with the formation of urea derivatives (carbamylation):

Protein-NHj + O = C = NH - »Protein-NH - CO-NH ₂

This leads to the fact that such solutions already in the course of the period of time which is required for the electrophoresis, new reaction products form, so that the result of the electrophoresis is then no longer unambiguous, because in addition compounds that were not initially present in the preparation appeared. In the case of completely delivered layers, it must be expected that these will be before Use for months and not even stored at refrigerated temperature. From the known equilibrium position and the kinetic data For the equilibrium according to equation (1), concentrations of up to 5 μπιοΐ / ΐ cyanate must be expected. On the other hand, it is known that already concentrations of 2.5 μΐηοΐ / l cyanate Hemoglobin at least 1 mole within the time required for electrophoresis Modify protein nitrogen according to equation (2) (see Fig. C).

In any case, layers which contain 50% urea can only be stored at room temperature. Is cooled to the common and also required refrigeration temperature of 0-4 ⁰ C., the urea crystallizes out and leads to irreversible changes in the layer. It is known that various derivatives of urea have similar, and in some cases even stronger, "chaotropic" effects, which result in the breaking of hydrogen bonds between the products. protein molecules: z. B. Baum, D. and Herkovits T. T. (1947) Biochemistry 13, 68-78.

The object of the present invention is now a properly working. Procedure for Analysis of protein subunits by means of electrophoresis, in which there is a risk of formation undesirable and the result falsifying reaction products is largely eliminated.

The solution to this problem is provided by the im

Characteristics of the claim conveyed technical teaching described.

The urea in layers of aqueous polyamide gel or agarose can according to the invention through Urea derivatives are substituted for those in water no cyanate ions form and which at lower Do not crystallize out at temperature. These are in particular alkyl-substituted ureas, namely the derivatives:

1 ¹ V ₄ I- "3 * -Γ» 4Γΐ9,

i \

N —CO —N

(3)

The advantage here is that such preparations in

significantly more dilute solution develop their dissociating properties, so that small amounts must be added. For example, with tetramethylurea, i.e. Ri - R4 = CH3, is already sufficient a concentration of 50 g / l to ensure complete dissolution in this state during electrophoresis to secure.

example 1

A polyester film expediently produced by polymerizing aliphatic diols and dicarboxylic acids is coated with an aqueous layer of polyacrylamide gel Modified insofar as tetramethylurea was added in liquid form to the monomer after 50 g / l will. The polymerization proceeds in a similar way to that of layers which do not contain tetramethylurea got added.

Example 2

An S-layer produced analogously to Example 1 is modified by adding 150 g / l Butyl urea can be added.

Example 3

In the preparation of an aqueous urea derivative of the formula (3) containing (tetramethylurea) Layer of polyacrylamide gel on a polyester film According to Example 1 with adhesion promoter, three percent by weight (based on on solids) of an ampholyte according to patent 21 37 617 admixed, in particular according to Example 5c of the patent specification produced cut between pH 6 and 6.9.

Example 4

On a tetramethylurea and ampholyte prepared according to Example 1 to 3 between pH 6 and 6.9 containing aqueous layer of polyacrylamide gel on a plastic film with an adhesion promoter samples of 5 μΐ of a solution of hemoglobin from a human were in an electrophoresis apparatus Newborns applied in 50% urea. For details see Altland, K. and Kaempfer, N. (1980) Electrophoresis 1, 57-62. They were subjected to electrophoresis.

Comparative experiment:

To prove the technical progress, three differently produced were in a comparative experiment thin layers of aqueous polyacrylamide gel on polyester films compared which contained the following additives:

A) 59% urea, freshly made,

B) 5% tetramethylurea, then 126 days

stored at 18 ° C

C) 50% urea, then stored at 18 ° C for 126 days.

All three layers were electrophoresed under uniform conditions according to Example 4 for the Globin fragments used in neonatal human blood The zones were photometry, with in reference is made to German patents 2127 617 and 23 30 743 for the details. From the Figures A-C (Figs. I-III) it can be seen that a Layer with urea content stored under unfavorable conditions, the dissolution of the globin components practically prevented, while the inventively stored under the same conditions with tetramethylurea produced layer compared to a layer freshly produced by the currently customary methods Urea-prepared layer does not differ, i.e. four months of storage at room temperature survives without impairment.

1 sheet of drawings

Claims (1)

Claim: Method for the analysis of protein subunits using electrophoresis on thin Layers using layers of aqueous polyacrylamide gels on polyester films, in particular by polymerizing aliphatic diols polyester films obtained with dicarboxylic acids, characterized in that the gels contain substituted urea derivatives, in which the free hydrogen molecules of urea are partially or completely replaced by alkyl radicals with straight or branched chains, which 1 to 4 Contains carbon residues.