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通过串联质谱分析鉴定猪肝酯酶变体及其特性研究。

Identification of pig liver esterase variants by tandem mass spectroscopy analysis and their characterization.

作者信息

Brüsehaber E, Böttcher D, Musidlowska-Persson A, Albrecht D, Hecker M, Doderer K, Bornscheuer U T

机构信息

Institute of Biochemistry, Department of Biotechnology & Enzyme Catalysis, Greifswald University, Felix-Hausdorff-Str. 4, 17487, Greifswald, Germany.

出版信息

Appl Microbiol Biotechnol. 2007 Sep;76(4):853-9. doi: 10.1007/s00253-007-1061-2. Epub 2007 Jun 26.

DOI:10.1007/s00253-007-1061-2
PMID:17593363
Abstract

Pig liver esterase (PLE) is probably the most important carboxyl esterase in organic synthesis and is commercially obtained by extraction of the animal tissue. However, problems occur in its application due to the presence of several isoenzymes (alpha-, beta- and gamma-PLE). The functional expression of the gamma-isoenzyme was already shown and differences in the enantioselectivity compared to the commercial preparations were confirmed. The amino acid and nucleotide sequences of the alpha- and beta-PLE are still unknown. In this work, putative sequences of the alpha-isoenzyme were identified from a commercial PLE preparation by 2D gel electrophoresis, digestion with proteases and analysis using Matrix-assisted laser desorption/ionization-time of flight (TOF) and electrospray ionisation quadrupole-TOF mass spectrometry. Based on these results, three amino acid exchanges were introduced into the gene encoding gamma-rPLE by site-directed mutagenesis, and the proteins were expressed in E. coli Origami (DE3). The produced PLE mutants were characterised with respect to their substrate specificity and enantioselectivity. No significant differences in the activity towards methyl butyrate were found, but several variants showed substantially enhanced enantioselectivity in the resolution of (R,S)-1-phenyl-2-butyl acetate with E = 100 for the best mutant V236P/A237G.

摘要

猪肝酯酶(PLE)可能是有机合成中最重要的羧酸酯酶,可通过提取动物组织进行商业获取。然而,由于存在几种同工酶(α-、β-和γ-PLE),其应用中出现了问题。γ-同工酶的功能表达已经得到证实,并且与市售制剂相比,对映选择性的差异也得到了确认。α-和β-PLE的氨基酸和核苷酸序列仍然未知。在这项工作中,通过二维凝胶电泳、蛋白酶消化以及使用基质辅助激光解吸/电离飞行时间(TOF)和电喷雾电离四极杆-TOF质谱分析,从市售PLE制剂中鉴定出α-同工酶的推定序列。基于这些结果,通过定点诱变将三个氨基酸交换引入编码γ-rPLE的基因中,并在大肠杆菌Origami(DE3)中表达蛋白质。对产生的PLE突变体的底物特异性和对映选择性进行了表征。发现对丁酸甲酯的活性没有显著差异,但几个变体在(R,S)-1-苯基-2-丁基乙酸酯的拆分中表现出显著增强的对映选择性,最佳突变体V236P/A237G的E值为100。

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