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通过定点诱变对红平红球菌KA2-5-1中参与二苯并噻吩脱硫途径的2'-羟基联苯-2-亚磺酸盐脱亚磺酶进行改进。

Improvement of 2'-hydroxybiphenyl-2-sulfinate desulfinase, an enzyme involved in the dibenzothiophene desulfurization pathway, from Rhodococcus erythropolis KA2-5-1 by site-directed mutagenesis.

作者信息

Ohshiro Takashi, Ohkita Ryo, Takikawa Takeshi, Manabe Masanori, Lee Woo Cheol, Tanokura Masaru, Izumi Yoshikazu

机构信息

Department of Biotechnology, Tottori University, Japan.

出版信息

Biosci Biotechnol Biochem. 2007 Nov;71(11):2815-21. doi: 10.1271/bbb.70436. Epub 2007 Nov 7.

DOI:10.1271/bbb.70436
PMID:17986771
Abstract

In the microbial dibenzothiophene desulfurization pathway, 2'-hydroxybiphenyl-2-sulfinate is converted to 2-hydroxybiphenyl and sulfinate by desulfinase (DszB) at the last step, and this reaction is rate-limiting for the whole pathway. The catalytic activity and thermostability of DszB were enhanced by the two amino acid substitutions. Based on information on the 3-D structure of DszB and a comparison of amino acid sequences between DszB and reported thermophilic and thermostable homologs (TdsB and BdsB), two amino acid residues, Tyr63 and Gln65, were selected as targets to mutate and improve DszB. These two residues were replaced by several amino acids, and the promising mutant enzymes were purified and their properties were examined. Among the wild-type and mutant enzymes, Y63F had higher catalytic activity but similar thermostability, and Q65H showed higher thermostability but less catalytic activity and affinity for the substrate. To compensate for these drawbacks, the double mutant enzyme Y63F-Q65H was purified and its properties were investigated. This mutant enzyme showed higher thermostability without loss of catalytic activity or affinity for the substrate. These superior properties of the mutant enzyme have also been confirmed with resting cells harboring the mutant gene.

摘要

在微生物二苯并噻吩脱硫途径中,2'-羟基联苯-2-亚磺酸盐在最后一步通过脱亚硫酸酶(DszB)转化为2-羟基联苯和亚磺酸盐,该反应是整个途径的限速步骤。两个氨基酸取代增强了DszB的催化活性和热稳定性。基于DszB的三维结构信息以及DszB与已报道的嗜热和耐热同源物(TdsB和BdsB)之间的氨基酸序列比较,选择两个氨基酸残基Tyr63和Gln65作为突变靶点以改进DszB。用几种氨基酸替换了这两个残基,对有前景的突变酶进行了纯化并检测了其性质。在野生型和突变酶中,Y63F具有较高的催化活性但热稳定性相似,而Q65H表现出较高的热稳定性但催化活性和对底物的亲和力较低。为了弥补这些缺点,对双突变酶Y63F-Q65H进行了纯化并研究了其性质。该突变酶表现出较高的热稳定性,同时不丧失催化活性或对底物的亲和力。携带突变基因的静息细胞也证实了该突变酶的这些优异特性。

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