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Co-expression of an organic solvent-tolerant lipase and its cognate foldase of pseudomonas aeruginosa CS-2 and the application of the immobilized recombinant lipase

机译:铜绿假单胞菌CS-2耐有机溶剂脂肪酶及其同源折叠酶的共表达及固定化重组脂肪酶的应用

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The genes of CS-2 lipase and its cognate foldase were cloned from Pseudomonas aeruginosa CS-2. A stop codon was not found in the lipase gene. The amino acid sequence deduced from the lipase gene from P. aeruginosa CS-2 showed 97.8%, 71.3%, and 71.2% identity with lipases from P. aeruginosa LST-03, P seudomonas mendocina ymp, and Pseudomonas stutzeri A1501, respectively. The co-expression of CS-2 lipase and its cognate foldase of P. aeruginosa CS-2 in E scherichia coli BL21 (DE3) resulted in the formation of a soluble lipase. The recombinant lipase and foldase were purified to homogeneity using nickel affinity chromatography and about 10.2-fold with 40.9% recovery was achieved for the purification of the recombinant lipase. The molecular masses of the lipase and the foldase were estimated to be 35.7 and 38.3 kDa in SDS-PAGE, respectively. The recombinant lipase showed stability in the presence of some organic solvents. The recombinant CS-2 lipase was immobilized and subsequently used for the synthesis of butyl acetate in heptane. The conversion of substrate decreased from 98.2% to 87.4% after 5 cycles in reuse of the immobilized lipase.
机译:从铜绿假单胞菌CS-2克隆了CS-2脂肪酶及其同源折叠酶的基因。在脂肪酶基因中未发现终止密码子。从铜绿假单胞菌CS-2的脂肪酶基因推导的氨基酸序列分别与铜绿假单胞菌LST-03,门氏假单胞菌ymp和斯氏假单胞菌A1501的脂肪酶具有97.8%,71.3%和71.2%的同一性。 CS-2脂肪酶及其铜绿假单胞菌CS-2的同源折叠酶在大肠杆菌BL21(DE3)中的共表达导致可溶性脂肪酶的形成。使用镍亲和层析将重组脂肪酶和折叠酶纯化至均质,并纯化重组脂肪酶,获得约10.2倍的回收率和40.9%的回收率。在SDS-PAGE中,脂肪酶和折叠酶的分子量分别估计为35.7和38.3 kDa。重组脂肪酶在某些有机溶剂存在下显示出稳定性。将重组CS-2脂肪酶固定,随后用于庚烷中乙酸丁酯的合成。在重复使用固定化脂肪酶的5个循环后,底物的转化率从98.2%降至87.4%。

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