A recombinant Pichia pastoris producing small molecule hyaluronic acid and its construction method
A Pichia pastoris and hyaluronic acid technology, applied in the field of recombinant Pichia pastoris and its construction, can solve the problems of expensive substrates, cumbersome steps, low synthesis efficiency and the like, and achieve the effects of reducing viscosity and being easy to purify and recover
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Embodiment 1
[0037] Cloning of embodiment 1hasA gene and UDP-glucose dehydrogenase tuaD gene
[0038] The hasA gene used in the present invention is derived from Streptococcus zooepidemicus ATCC 35246 and the UDP-glucose dehydrogenase gene is derived from Bacillus subtilis. The Streptococcus zooepidemicus strain is inoculated with 5ml of M17 liquid medium and cultured at 37°C and 200rpm for 16h. Bacillus subtilis was inoculated in 5ml LB liquid medium and cultured at 37°C and 200rpm for 16h. Pichia pastorisGS115 was inoculated in 5ml YPD liquid medium, cultured at 200rpm and 30°C for 24h. Bacteria were collected separately, and the genomic DNA of the three strains was extracted using a bacterial genome extraction kit.
[0039] According to the published genome information sequence, design primers hasA-F / hasA-R, tuaD-F / tuaD-R respectively, use the extracted genomic DNA as a template, and use standard PCR amplification system and program to amplify and obtain hasA respectively and tuaD gen...
Embodiment 2
[0049] Construction of embodiment 2 recombinant plasmid PAPT9K
[0050] The amplified DNA fragments hasA, tuaD, GAP and TEF1 were used to fuse the promoter and the target gene by fusion PCR respectively. The specific operation procedure is as follows: take 2 ul of hasA and GAP fragments and mix them in a PCR tube, add 21 μl of sterile water and 25 μl of 2xsuper pfu Master Mix (Hangzhou Baosai Biotechnology Co., Ltd.), mix well, place in a PCR instrument, and run according to the following procedures: 94°C for 3min, [94°C for 30s, 50°C for 30s, 72°C for 1min]×10, 72°C for 5min. Immediately after self-fusion PCR without primers, add 1 μl of primers gap-F and hasA-R, mix well and run according to the following program: 94°C for 3 minutes, [94°C for 30s, 55°C for 30s, 72°C for 1min]×32,72 ℃ 5min. After the PCR product was subjected to 1% agarose gel electrophoresis, the target band was recovered by cutting the gel to obtain the GAP-hasA fragment.
[0051] Similarly, the TEF1-tu...
Embodiment 3
[0052] Embodiment 3 The strain construction of recombinant Pichia pastoris producing HA
[0053] After the recombinant plasmid PAPT9K was linearized with SalI, according to the operation manual of Pichia pastoris, the Pichia pastorisGS115 host was electroporated, and positive recombinants were screened with MD plate (histidine-deficient selection marker). At the same time, in order to screen for hosts with multi-copy insertions, high-copy screening was performed on YPD plates containing different concentrations of antibiotic g418. The fermented recombinant strain used in the present invention is a positive recombinant strain screened out at 4 mg / ml, named PAPTGS115.
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