[beta]-mannase heat-resistant mutant M14, recombinant bacterium and application thereof
A technology of mannanase and mutants, which is applied in the fields of genetic engineering and enzyme engineering, can solve the problems of unstable biological activity and heat resistance that cannot meet industrial requirements, and achieve the effects of optimizing charge distribution and improving heat resistance
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Embodiment 2
[0055] 6. Example 2: Construction of β-mannanase site-directed mutant recombinant vector
[0056] Using the recombinant vector pPICZαA-ManAK containing the ManAK gene as a template, add primers for the mutation site, and perform PCR amplification with high-fidelity enzymes. The product is digested with DpnⅠ and transformed into DH5α E. Positive clones were screened on the LB plate, and the sequencing work was completed by Qingdao Ruibo Xingke Co., Ltd.
Embodiment 3
[0057] 7. Example 3: Construction of β-mannanase site-directed mutant expression vector
[0058] The positive clones with correct sequencing after mutation in Example 2 were extracted and purified, and the corresponding plasmids were linearized with Sac I single enzyme digestion, electrotransformed into Pichia pastoris X33, and screened on MD plates to obtain the transformants of each mutant expression strain. Transfer to YPD plate for activation.
Embodiment 4
[0059] 8. Example 4: Verification of high-throughput expression of β-mannanase mutants in Pichia pastoris
[0060] Pick the activated transformant in Example 3 and inoculate it into 1mL of BMGY medium, culture it in a 48-well plate at 30°C and 200rmp on a shaker, add 1% methanol of the culture volume for the first time after 24h to induce the expression of the enzyme, and then the culture process Induced once every 24h. After inducing expression for 96 hours, the culture medium was centrifuged to obtain the supernatant, and the activity and thermal stability of β-mannanase in the fermentation medium supernatant were determined.
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