DD274447C2 - PROCESS FOR PRODUCING DEFINED PROTEINS - Google Patents

Description

Field of application of the invention

The invention relates to a process for the production of defined proteins with the aid of genetically modified microorganisms. Field of application of the invention is the microbiological industry.

Characteristic of the known technical solutions

It has long been known that genes from animals, plants, prokaryotes and viruses can be expressed by genetic engineering methods. This opens up the possibility of microbially producing special proteins of these organisms. Particularly noteworthy are the examples human insulin (DD-AP 155004), interferon (DD-AP 202085, DD-AP 202307, DD-AP 160280), human growth hormone (DD-AP 202045, DD-AP 202046) and various microbial enzymes. The vectors used are plasmids and their derivatives as well as bacteriophages and their derivatives. As hosts in which these vectors are replicated and genes are primed, Escherichia coli, Bacillus subtilis and Saccharomyces cerovisiae have been most commonly used.

A disadvantage of the methods developed so far is that complex and expensive media are used. As carbon sources, carbohydrates are usually used; the media have a neutral pH. These factors promote contamination by other microorganisms. They require strict sterility control of the process and make it difficult to carry out continuous cultivation and mass production. It is therefore the application of protective carbon sources and simple media such. As methanol and simple mineral salt solutions sought. One expression of this is host-vector systems which include methylotrophic bacteria (GB-PS 2003926, EP 0066994). The disadvantage of the previously known systems with methylotrophic bacteria, however, is that the growth optimum of the hosts in the neutral pH range, whereby they are also exposed to the competition of a variety of Kontaminantun, developing, for example, as substrate competitors or as secondary flora on the fermentation products formed can. Another disadvantage of such hosts, such as E. coli, is that product formation is associated with toxin formation, requiring elaborate measures to separate the toxin from the product.

Object of the invention

The object of the invention is to provide host-vector systems capable of exploiting such substrates with protective action such as methanol, growing on simple mineral salt solutions, and protecting by a pH optimum of the growth in the acidic region for the recovery of defined proteins to achieve contamination. By introducing such

Host vector systems are being created for industrial mass production. In addition, the hosts to be used are those microorganisms which are non-pathogenic and toxin-free, which is important not only in terms of occupational safety and general safety in the production process, but also in terms of simplified processing of the product.

Explanation of the essence of the invention

The essence of the invention is that host-vector systems are used for the production of proteins of animal, plant, microbial or viral origin in which the hosts are acidophilic methanol oxidizing or methanolutilizing bacteria. These bacteria belong preferably to the genera Acetobacter and Gluconobacter. The methylotrophy is optional. Preferred hosts according to the invention are strains of the species Acetobacter methanolicus, which are distinguished by methylotropnia in combination with a pronounced acidophilicity and, in comparison to other acetobacteria, high reproductive capacity. The pH optimum for growth is 3.8-4.0. The bacteria of this group are non-pathogenic and toxin-free. As basis vectors for the realization of the invention known Klonierungsvektoren, Plat, aide of the kinds Acetobacter and Gluconobacter or phages of the kinds Acetobacter and Gluconobacter are used.

Hasmids of the incompatibility groups Ine P1 and Inc P4 (B. B. RP4, R68.45 and RSF1010) and their derivatives on the one hand and plasmids of strains of the genera Acetobacter or Gluconobacter on the other hand are preferably used. According to the invention, virulent and temperate phages of Acetobacter or Gluconobacter, preferably of Acetobacter methanolicus, are used as further vectors. This applies, for example, phages M01, MO2, MO5 and MO6. Furthermore, known cloning vectors, for example pBR322, are used for the construction of hybrid plasmids with the vectors listed above.

The construction of the vectors and the gene transfer are carried out according to known methods, as substrates for dio fermentation methanol and / or substances with C-C bonds are used. Preferred substances with C-C bonds are ethanol, glucose, glycerol or acetic acid.

By the method according to the invention, the intended objectives are achieved. It allows the formation, accumulation and recovery of defined proteins from methanol or substrates with C-C bonds through microbial fermentation. Such proteins may be insulin, interferon, chymosin, PLV protein as well as intracellular and extracellular microbial enzymes. The accumulation of intracellular enzymes can be carried out with the aim of overproduction of certain metabolites (ζζΒ amino acids, organic acids, vitamins) or the optimization of metabolic pathways (verbesserte Β., Improved yield coefficients in fermentations, extension of the substrate spectrum). The invention will be explained in more detail with the following examples.

Embodiment 1

Production of gene products (proteins) by expression of alien antibiotic resistance genes into the methanolutilislerenden strain Acetobacter methanolicus IMET B 346

1.1. Brief description of the strain Acetobacter methanolicus IMET B 346

Acetobacter methanolicus IMET B346 is a strain of the newly described bacterial species Acetobacter methanolicus. He was deposited in the culture collection of the Central Institute for Microbiology and Experimental Therapy Jena of the AdW of the GDR.

The strain was isolated from a yeast fermentation process with methanol as sole carbon and energy source.

It is acidophilic and facultative methylotrophic. Unlike other Acetobacter strains, IMET B 346 shows good growth on methanol, glucose, gluconic acid, 2,3-butanediol and caproic acid as the sole source of carbon and energy. For growth, pantothenic acid or yeast extract is needed.

DNA-rRNA hybridization experiments confirm that they belong to Acetobacter. The incorporation of methanol takes place via the hexulose phosphate pathway. The GC content of the strain is 62.3 mol%.

A preferred culture medium has the following composition (mg / l):

NH ₄ CI-761.4; CaCl ₂ · 6H ₂ O - 5.47; MgSO ₄ .7H ₂ O - 71.2; ZnSO ₄ 7H ₂ O - 0.44; MnSO ₄ .4H ₂ O - .775; CuSO ₄ .5H ₂ O-0.785; Na ₂ MoO ₄ .2H ₂ O - 0.252; FeSO ₄ .7H ₂ O - 4.98; KH ₂ PO _{4 to} 68.05; K ₂ HPO ₄ - 87.09, pantothenic acid -10, methanol -1 vol .-% to 1 liter of distilled water. It is adjusted pH4.0.

1.2. Conjugative transfer of plasmid 3 R68.45 into strain IMET B346 and expression of Pseudomonas antiblotic residues in this strain Plasmid Π68.45 (Haas and Holloway, 1976) belongs to the IncPI incompatibility group of Pseudomonas.

R 68.45 (37.5 Md) encodes tetracycline, kanamycin and carbenicillinresity.

The donors used are the strains Pseudomonas PAD ML 4262 (Sagai et al., 1975) and Escherichia coli SK 1590 (Kushner, 1978) into which the plasmid R68.45 was conjugatively transferred. The conjugative transfer of the plasmid from the neutrophil strains into the acidophilic methylotrophone strain IMET B346 is hampered by the different pH optima for growth.

In growth experiments it was determined that at pH = 6, the cultivation of both the neutrophils and the acidophilic strain is possible.

For the conjugation experiments, an agar (pH = 6) stabilized with Sörensen phosphate buffer is used, which in addition to the in 1.1. specified trace salts 1% methanol, 0.1% glucose, 20μς / ητιΙ pantothenic acid and 20ng / ml thiamine (in crosses with E. coli SK1590 (R68.45) or 50 \ ig / m \ tryptophan, isoleucine, valine and methionine (at crosses with Ps. aeruginosa ML 4262 (R68.45) and 1.8% agar-agar.

Donor and recipient are his grown to a cell density of about 10 "cells / ml and the ratio of 1:.. 0.2 ml of the mixture are mixed for 3 spatulated on Konjugationsplatten with the above-described agar After 24 hours of incubation at 3O ⁰ C, the cells are in 2ml of Sörensen buffer was sampled on Selsktionsplatten for detection of the Transkonjugenten (selection on Tetracycline Residue-6 (^ g / mlTetrazyklln) and for titer determination of donor and Reziplent.) The transconjugants are checked for the simultaneous acquisition of other antibiotic resistance markers of the plasmid (kanamycin, carbenicillin).

The transfer of the plasmid R68.45 from the strains Ps.aeruglnosa ML4262 (R68.45) or E. coli SK1590 (R68.45) takes place with a frequency of 10 ² or about 10 ~ ⁴ transconjugants per recipient cell into the strain IMET B346.

Of every 100 transconjugants tested, all are normally resistant to kanamycin (200 μg / ml) and carbenicillin (2QQ0 \ ig / m \) , while the strain IMET 8346 is not capable of growth at these antibiotic concentrations .

The ability to conjugate the plasmid is checked by conjugations between the plasmid-bearing transconjugant IMET B346 (R68.45) and a rifampicin-resistant mutant of this strain. The selection medium contains Tetra2yklin (50pg / ml) and rifampicin (50pg / ml). Tetracycline-resistant transconjugants occur at a rate of 10 ^{-3 3} -10 ⁵ per donor cell as a function of the plasmid-bearing donor, and the transconjugants simultaneously acquire kanamycin and carbenicillin resistance.

It is also the reverse transfer of R68.45 from IMET B346 (R68.45) in the strains Ps. Aeruginosa ML4262 and E. coli C600 possible. The selection is based on tetracycline resistance, for counterselection rifampicin is used. The transfer rates of the plasmid are about 10 "transconjugants per recipient (in crosses with Ps.aeruginosa ML4262) and about 10" ⁴ transconjugants per recipient cell (in crosses with E. coli C600). The transconjugants acquire kanamycin and carbenicillin resistance simultaneously.

The simultaneous conjugative transfer of various plasmid markers (antibiotic resistance, origin of replication, Tra genes) shows that the plasmid R 68.45 is completely transferred to the strain IMET B346. The antibiotic resistances that occur prove that the responsible gene products (e.g., β-lactamase, phosphotransferase) are synthesized by expression of the Pseudomonas antibiotic resistance genes in the methylotrophic bacterium.

1.3. Mobilization of the plasmid RSF1010 by means of R68.45 by conjugation into the strain Ac. methanolicus IMET B346 and expression of the Escherichia coli Streptomycin resistance gene in this strain The plasmid RSF1010 (Guerry et al., 1974) belongs to IncQ Incompatibility Group; (lncP4 from Pseudomonas) and determines streptomycin resistance. It is not transmissibly conjugative, but can be mobilized by other plasmids (eg R68.45).

For mobilization, Pseudomonas aeruginosa PAO ML 4262 (RSF1010, R68.45) and Escherichia coli SK1590 (RSF 1010, R 68.45) are used as donor strains.

Doncr and recipient are cultured to a cell density of about 10 ⁸ -10 ⁹ cells / ml and mixed in a ratio of 1: 5. 0.2 ml of the mixture are applied to conjugation plates having the same composition as in 1.2. have, spat. After 24 hours incubation at 30 ° C, the cells are taken up in 2 ml Sörensenpuffer and herauspatelt on selection plates.

The selection plates contain in addition to the 1.1. described medium with 1.8% agar supplement still 50pg / ml tetracycline (selection on R68.45 transfer), 200pg / ml streptomycin (selection on RSF1010 transfer) or both antibiotics (selection for transfer of both plasmids). At the same time, live cell count determinations are performed on donor and recipient on appropriate selective media and controls for detecting antibiotic-resistant mutants.

The transfer rates of the Pasmids RSF1010 be at intersections using Ps.aerugionosa ML4262 (RSF1010, R 68.45) about 10 ~ ² transconjugants per donor cell, wherein crosses using E. coli SK1590 (RSF 1010 R 68.45) about 10 ~ ⁴ transconjugants per donor cell. The corresponding transfer rates of the plasmid R68.45 are about four times higher in both crosses. Approximately 10-20% of the RSF1010-bearing transconjugants simultaneously contain R68.45.

Resistance to streptomycin in IMET B346 (RSF 1010) proves that the responsible gene product (phosphotransferase) is synthesized by expression of the Escherichia coli antibiotic resistance gene in the methylotrophic bacterium.

literature

Guerry, P., J. VanEmbden, S. Falkow, 1974.

J. Bacteriol. 117: 619-630.

Haas, D., B.W. Holloway, 1976.

Molec. Gene. Genetics 144: 243-251.

Kushner S.S., 1978.

In: Genetic Engineering (H.VV. Boyer, S. Nicosia, ed.), Elsevier / North-Holland, pp. 17-23.

Sagai, H., V.Kremen /, K.Hasuda, S.lyobe, H.Knothe, S.Mitsuhashi, 1975, Jpn. J.Microbiol. 19: 427-432.

Example 2

Production of the phage vector

By fermentation of strain MB70 on methanol as sole carbon and energy source, culture filtrates were generated and 2 phage strains were isolated with differing host spectra. The phages were designated MO 5 and MO 6.

Both phages are capable of lysogenizing the sensitive MB70 strain:

Genetic material (phage genome) is introduced with the phage MO5 in the acidophilic methanolassimilierenden MB70 bacterial strain. The phage MO5 contains double-stranded DNA and proliferates virally on strain MB70 with a latency of 90 minutes and a litter size of 58 pfu / ml of infected cell. For the introduction of the phage genome in the host cell (lysogenization) are equal proportions of a suspension of the bacterial strain (about 10 ⁹ cfu / ml) and a

Suspension of phage MO5 (about 10 ⁹ pfu / ml) mixed and herauspatelt on Grundagarplatten. After an incubation period of 3 to 4 days, the surviving colonions are isolated and tested for sensitivity to the phage MO 5. Selected M05-insensitive isolates are grown in submerged culture and irradiated with UV light to induce the lytic cycle of the introduced prophage. The starting material for the induction experiments were exponentially grown submerged cultures of the MO5 lysogenized strain MB70.

The UV irradiation of the bacterial suspension was carried out in Petri dishes (bed height 0.2 cm) under a low-pressure mercury vapor lamp having an emission maximum at 253,7nm in the dose range between 250 and 3000erg · mm ^'1. For all examined MO5-resistant isolates could be a release of phage MO5 can be achieved by UV irradiation of the lysogenized host cells.

According to the principle explained in the example for the isolation of phage vectors from the MB70 strain, further vectors can be isolated from other acidophilic r. Ethanol-utilizing bacterial strains (desires et al., Z.Allg.Mikrobiol., 23 [2] 1983, 81 to 94).

Claims (9)

1. A process for the preparation of defined proteins by recombination of a DNA sequence with a vector, transfer of the resulting recombinants in a microorganism and subsequent fermentation, characterized in that as hosts acidophilic methanol oxidizing or methanolutibisierende bacteria, known as base vectors cloning vectors, plasmids of the genera Acetobacter and Gluconobacter or phages of the genera Acetobacter and Gluconobacter and used as substrates methanol and / or substances with CC bonds. 2. The method according to claim 1, characterized in that bacteria are used as hosts of the genera Acetobacter and Gluconobacter. 3. The method according to claim 1 and 2, characterized in that are used as hosts strains of the species Acetobacter methanolicus. 4. Process according to Claims 1 to 3, characterized in that the strains IMET10945 or IMET B 346 or Acetobacter methanolicus MB 70 are used as hosts. 5. The method according to claim 1, characterized in that are used as vectors plasmids of incompatibility groups IncPI and Ine P4, such as RP4, R68.45 and RSF1010 and their derivatives. 6. The method according to claim 1, characterized in that are used as vectors plasmids of strains of the genera Acetobacter or Gluconobacter. 7. The method according to claim 1, characterized in that are used as vectors phages of Acetobacter methanolicus, such as MO 1, MO2, MO5 and MO6. 8. The method according to claim 1, characterized in that hybrids from known cloning vectors and the vectors according to claim 6 and 7 are used as vectors. 9. The method according to claim 1 to 8, characterized in that are used as substances with C-C bonds, ethanol, glucose, glycerol or acetic acid.