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耐热赖氨酸氨肽酶毕赤酵母表达及培养条件优化
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Expression and Optimization Thermo-Stable Lysine Aminopeptidase inP. pastoris
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DOI:10.3969/j.issn.1673-1689.2018.06.004
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中文关键词: 关键字: 铜绿假单胞杆菌 耐热氨肽酶 基因克隆 培养条件优化
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英文关键词: Pseudomonas aeruginosa,thermo-stable aminopeptidase,gene cloning,optimization of culture condition
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基金项目:
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中文摘要:
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为实现耐热耐氨酸氨肽酶的异源表达,通过PCR扩增技术从Pseudomonas aeruginosa NJ -814基因组中克隆获得耐热的赖氨肽酶基因(PLAP),构建重组载体pPIC9K-PLAP,并最终实现在毕赤酵母GS115中的分泌表达。对重组毕赤酵母进行初步筛选,单因素实验优化获得重组毕赤酵母最佳诱导条件如下:诱导培养基初始pH为5.0、甲醇质量浓度1.5 g/dL、诱导温度28 ℃、装液量25 mL/250 mL、Co2+浓度50 μmol/mL、山梨醇添加量9 g/L。在最优条件下,氨肽酶酶活提高了5.2倍,比酶活2.74 U/mg。实验结果表明:PLAP基因已成功转入毕赤酵母GS115并获得表达。
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英文摘要:
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The aim of this study was toachieve heterologous expression of thermo-Stable Lysine Aminopeptidase(PLAP),the PLAP gene thathave been investigated producing a thermo-stable Lysine Aminopeptidasewas cloned from the genomic DNA of Pseudomonas aeruginosa NJ-814 by PCR.The expression vector pPIC9K-PLAP was constructed to express extracellular protein in P. pastoris GS115. After preliminary screening of the recombinant P. pastoris,the optimized fermentation conditions based on single factor experiment wereidentified as follows:induction methanol concentration was 15 g/L,induction pH was 5.0,induction temperature was 28 ℃,the medium volume was 25 mL/250 mL,the amount of Co2+ was 50 μmol/mL,induction sorbitol was 9 g/L. Finally,the enzyme activity was 5.2 times as in original conditions,the specific activitywas 2.74 U/mg. The result showed that PLAP gene has been successfully transferred and expressed in the Pichia pastoris GS115。
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