Efficient Production of Active RecombinantCandida rugosaLIP3 Lipase inPichia pastorisand Biochemical Characterization of the Purified Enzyme

毕赤酵母 皱纹假丝酵母 重组DNA 脂肪酶 分子生物学 密码子使用偏好性 重叠延伸聚合酶链反应 生物 基因 毕赤酵母 基因亚型 生物化学 限制性酶 表达式向量 基因组
作者
Shu‐Wei Chang,Guan-Chiun Lee,J. F. Shaw
出处
期刊:Journal of Agricultural and Food Chemistry [American Chemical Society]
卷期号:54 (16): 5831-5838 被引量:40
标识
DOI:10.1021/jf060835e
摘要

Candida rugosa lipase (CRL), an important industrial enzyme, possesses several different isoforms encoded by the high-identity lip gene family (lip1 to lip7). In this study, an additional N-terminal peptide in front of the lip3 gene was removed by PCR, and the 18 nonuniversal serine codons (CTG) of the lip3 gene were converted into universal serine codons (TCT) by means of an overlap extension PCR-based multiple-site-directed mutagenesis to express an active recombinant LIP3 in the yeast Pichia pastoris. The regional synthetic DNA fragment (339 bp) is first recombined by primer assembly with 20 overlapping nucleotides, followed by specific overlap extension PCR with outside primers containing restriction enzyme sites for directional cloning into the pGAPZalphaC vector. The results show that the production yield (0.687 unit/mL) of N-fused lip3 (nflip3) has an overall improvement of 69-fold relative to that (0.01 unit/mL) of lip3 and of 52-fold (0.47 unit/mL) of codon-optimized lip3 (colip3) relative to that (0.01 unit/mL) of non-codon-optimized lip3 (lip3), with the cultivation time set at 5 days. This finding demonstrates that the reservation of the N terminus and the regional codon optimization of the lip3 gene fragment at the 5' end can greatly increase the expression level of recombinant LIP3 in the P. pastoris system. The purified recombinant LIP3 shows distinct biochemical properties compared with other isoforms.
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