DD265164A1 - PROCESS FOR PREPARING PROTEINOGENIC ACTIVE SUBSTANCES - Google Patents

Abstract

The invention includes a method for producing proteinogenic drugs. The invention relates to a method with which, above all, enzymes can be produced on a large scale and without much effort. Instead of microorganisms are used as genetically engineered organisms simply higher plants that are reproducible in field crops. For this purpose, a DNA sequence coding for the corresponding enzyme is coupled with appropriate promoters and the gene thus formed is integrated into the genome of the plants. From the regenerated, propagated, grown and harvested plants, the enzyme is obtained, whereby all the proteins that do not interfere with the application of the enzyme, must not be removed. The invention is particularly suitable for the production of chymosin.

Description

Field of application of the invention

The invention relates to a method for producing proteinogenic active substances using genetically engineered organisms.

Characteristic of the known state of the art

For the production of industrially or medically usable enzymes and other proteinogenic active substances (eg hormones), genetically manipulated microorganisms are increasingly being used. Such biotechnological production processes are of great economic importance, in particular, if the organisms in which the active substance in question naturally occurs are limited in size! Scope available or are not suitable for the recovery of the active ingredient. For example, chymosin, which is indispensable as a milk clotting enzyme for the cheese industry, is traditionally isolated from the abomasum of slaughtered calves and is therefore available only in limited quantities. By transferring a coding for chymosin (or prochymosin) DNA sequence into suitable microorganisms (bacteria, yeast, fungi), it has now become possible to produce chymosin also biotechnologically, as described, inter alia, in PCT patent application 8500382 or in the EP patent applications 133756 and 154351 has been proposed. The genetically engineered microorganisms are cultured in fermentors and look id in the prochymosin in the culture liquid, which is then worked up to the finished product of the enzyme preparation. The fermentor technology is relatively expensive; In addition, the nutrient media required for fermentation can generally not be prepared with cheap waste products (eg molasses), but use carbohydrate and protein sources which are also suitable for human consumption and are therefore lost.

In principle, the same characteristics are proposed for the genetically engineered biosynthesis of other proteinogenic drugs proposed methods. All previously known such methods use microorganisms and accordingly require relatively expensive fermentors and nutrient media.

Object of the invention

The object of the invention is, in addition to the special case of chymosin, to provide enzymes or other proteinogenic active substances, especially those which are required in large quantities, in an easy-to-handle and economically favorable process, with only requirements being generally imposed on their purity as they are indispensable for their industrial use.

Explanation of the essence of the invention

Accordingly, the object of the invention has been to obtain proteinogenic agents by means of genetically engineered organisms without fermenters and expensive nutrient media would have to be used. According to the invention the object is achieved in that a cloned DNA sequence encoding a proteinogenic agent is coupled with such control sequences that ensure their expression in higher plants that the chimeric gene thus formed is integrated into the genome of plant cells in that whole plants are regenerated from the transformed plant cells and these are propagated and that the active ingredient preparations are obtained from the harvested plants. It is advantageous if the DNA sequence encodes an industrially or pharmaceutically used enzyme, for example a protease. The invention is particularly adapted to the cases in which the DNA sequence codes for calf-specific pre-prochymosin or prochymosin. It is also possible; that the DNA sequence encodes a non-enzymatic drug.

By the invention, the disadvantages of the previously known and used manufacturing processes are largely avoided. The cultivation of genetically manipulated plants such as tobacco can be done with conventional agricultural techniques and does not require expensive nutrient media. As an energy source for biological synthesis, the sunlight is used directly.

The process steps according to the invention can of course be varied in many ways without departing from the scope of the invention, as will be described in detail below.

It is immaterial to the invention how the DNA sequence encoding the desired drug is isolated and identified. Both natural DNA sequences from other organisms as well as genetically modified or synthetic DNA sequences can be used. It is also not excluded that it is a plant DNA sequence from which additional copies are integrated into the genome of the plant to increase the product yield. In the special case, a clone coding for prochymosin cDNA clone, which was obtained from the RNA of Kälberrnagsr.s worked.

To make the coding DNA sequence expressable in plant cells, it is coupled with a plant promoter, a plant polyadenylation sequence and optionally additional expression enhancing control sequences. The promoter can be constitutive or regulatable. For example, the promoter of the TR 2 'gene from the Ti plasmid of Agrobacterium tumefaciens is well suited. This promoter, which is a high constitutive

Level of expression in tobacco and other higher plants, is present in E. coli plasmids and has already been used to express bacterial genes in higher plants / 1, II.

So far, however, such chimeric genes have not been constructed with the promoter of the TR 2 'gene or with other plant-specific promoters, which code for prochymosin or another industrially usable drug.

It is essential to the invention that the biosynthesis of the desired active ingredient takes place in a suitable for field cultivation higher plant, sio is therefore not on the particularly favorable tobacco Nicotiana tabacum - limited.

The methods for the transfer of the gene, for the regeneration of whole plants from the transformed plant cells and for the propagation of the regenerated plants are arbitrary. According to the current state of knowledge, the desired result in many dicotyledonous plants can be achieved particularly advantageously by agrobacterium-mediated gene transfer / 2,3,4 /. It is important that (to increase the product yield also several copies of the chimeric gene can be integrated into the genome and that a hereditary stable transgenic plant stem is produced, which can be arbitrarily propagated.The procedure is such that in a larger number of transgenic Of the plants with the highest prochymosin content, progeny are then obtained by self-pollination, which are subjected to a renewed selection for high procchymosin production to increase through new gene transfer even further.

The active substance preparation is expediently obtained by extraction-for example of the tobacco leaves. Methods for large-scale extract extraction from vegetative plant material are known in principle. However, it can not be ruled out that occasionally dispenses with the extraction and the dried and crushed plant material can already be used as an enzyme preparation.

In view of the fact that the invention relates essentially to a combination of known per se and in other context already used process steps, the professional execution of which requires no further explanation in detail, can be dispensed with the disclosure of an embodiment.

literature

IM Veiten, J., Volten, L., Hain, R., Schell, J., EMBO J. 3 (1 £ 84) p.2723ff.

121 Vaeck, M., Reynaerts, A., Hoofte, H. Jansen, S., Oe Beuckeleer, M. Dean, C., Zabeau, M., Van Montagu, M., Leemans, J., Nature 328 ( 1987)

l'il Gheysen, G., Dhaese, P., Van Montagu, M., Schell, J., in "Genetic Flux In Plants" (ede. Hohn, R., Dennis, ES), pp 11-17, New York 1985 IA / Muller, AJ, Almond, RR, Schiemann, J., Simoens, C. Inze, D., Mol. Gen. Genet., 207 (1987), p.

Claims (5)

1. A process for the production of proteinogenic agents using genetically engineered organisms, characterized in that A coupled DNA sequence coding for a proteinogenic agent is coupled with those control sequences which ensure their expression in higher plants, - the chimeric gene thus formed is integrated into the genome of plant cells, - regenerated whole plants from the transformed plant cells and these are propagated and - The proteinogenic agents are obtained from the harvested plants. 2. Process according to claim characterized in that the DNA sequence encodes an industrially or pharmaceutically usable enzyme. 3. The method according to claim 1 and 2, characterized in that the DNA sequence encodes a protease. 4. The method according to claim 1 to 3, characterized in that the DNA sequence for calf-specific pre-prochymosin or prochymosin encodes. 5. The method according to claim 1, characterized in that the DNA sequence encodes a non-enzymatic active ingredient.