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β-内酰胺酶I的定点诱变与底物诱导失活

Site-directed mutagenesis and substrate-induced inactivation of beta-lactamase I.

作者信息

Thornewell S J, Waley S G

机构信息

University of Oxford, Sir William Dunn School of Pathology, U.K.

出版信息

Biochem J. 1992 Dec 15;288 ( Pt 3)(Pt 3):1045-51. doi: 10.1042/bj2881045.

Abstract

The substrate-induced inactivation of beta-lactamase I from Bacillus cereus 569/H has been studied. Both the wild-type enzyme and mutants have been used. The kinetics follow a branched pathway of the type recently analysed [Waley (1991) Biochem. J. 279, 87-94]. The substrate cloxacillin (a penicillin) formed an acyl-enzyme (characterized by m.s.), and it was probably the instability of this intermediate that brought about inactivation. A disulphide bond was introduced into beta-lactamase I (the wild-type enzyme lacks this bond) by site-directed mutagenesis: Ala-77 and Ala-123 were replaced by cysteine. Spontaneous oxidation yielded the disulphide. The activity of this newly cross-linked enzyme was a little diminished, but the stability towards inactivation by cloxacillin was not increased. A second mutant of beta-lactamase I was studied: this mutant lacked the first 17 residues, i.e. the first alpha-helix. The mutant had reduced activity towards ordinary (non-inactivating) substrates and no hydrolysis of cloxacillin could be detected. These mutant enzymes were expressed in Bacillus subtilis, and were purified from the extracellular medium.

摘要

对蜡样芽孢杆菌569/H的β-内酰胺酶I的底物诱导失活进行了研究。使用了野生型酶和突变体。动力学遵循最近分析的[Waley(1991) Biochem. J. 279, 87 - 94]类型的分支途径。底物氯唑西林(一种青霉素)形成了酰基酶(通过质谱表征),可能是这种中间体的不稳定性导致了失活。通过定点诱变将二硫键引入β-内酰胺酶I(野生型酶缺乏此键):将丙氨酸-77和丙氨酸-123替换为半胱氨酸。自发氧化产生二硫键。这种新交联酶的活性略有降低,但对氯唑西林失活的稳定性并未增加。研究了β-内酰胺酶I的第二个突变体:该突变体缺少前17个残基,即第一个α-螺旋。该突变体对普通(非失活)底物的活性降低,并且未检测到氯唑西林的水解。这些突变酶在枯草芽孢杆菌中表达,并从细胞外培养基中纯化。

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Mechanism of substrate-induced inactivation of beta-lactamase I.底物诱导β-内酰胺酶I失活的机制。
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