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活性位点残基酪氨酸55和酪氨酸114在白喉棒状杆菌C-S裂解酶催化作用和底物特异性中的作用

Role of active-site residues Tyr55 and Tyr114 in catalysis and substrate specificity of Corynebacterium diphtheriae C-S lyase.

作者信息

Astegno Alessandra, Allegrini Alessandra, Piccoli Stefano, Giorgetti Alejandro, Dominici Paola

机构信息

Department of Biotechnology, University of Verona, Strada Le Grazie 15, Verona, Italy.

出版信息

Proteins. 2015 Jan;83(1):78-90. doi: 10.1002/prot.24707. Epub 2014 Nov 18.

DOI:10.1002/prot.24707
PMID:25354840
Abstract

In recent years, there has been increased interest in bacterial methionine biosynthesis enzymes as antimicrobial targets because of their pivotal role in cell metabolism. C-S lyase from Corynebacterium diphtheriae is a pyridoxal 5'-phosphate-dependent enzyme in the transsulfuration pathway that catalyzes the α,β-elimination of sulfur-containing amino acids, such as L-cystathionine, to generate ammonia, pyruvate, and homocysteine, the immediate precursor of L-methionine. In order to gain deeper insight into the functional and dynamic properties of the enzyme, mutants of two highly conserved active-site residues, Y55F and Y114F, were characterized by UV-visible absorbance, fluorescence, and CD spectroscopy in the absence and presence of substrates and substrate analogs, as well as by steady-state kinetic studies. Substitution of Tyr55 with Phe apparently causes a 130-fold decrease in K(d)(PLP) at pH 8.5 providing evidence that Tyr55 plays a role in cofactor binding. Moreover, spectral data show that the mutant accumulates the external aldimine intermediate suggesting that the absence of interaction between the hydroxyl moiety and PLP-binding residue Lys222 causes a decrease in the rate of substrate deprotonation. Mutation of Tyr114 with Phe slightly influences hydrolysis of L-cystathionine, and causes a change in substrate specificity towards L-serine and O-acetyl-L-serine compared to the wild type enzyme. These findings, together with computational data, provide useful insights in the substrate specificity of C-S lyase, which seems to be regulated by active-site architecture and by the specific conformation in which substrates are bound, and will aid in development of inhibitors.

摘要

近年来,由于细菌甲硫氨酸生物合成酶在细胞代谢中起关键作用,其作为抗菌靶点受到了越来越多的关注。来自白喉棒状杆菌的C-S裂解酶是转硫途径中一种依赖于5'-磷酸吡哆醛的酶,它催化含硫氨基酸(如L-胱硫醚)的α,β-消除反应,生成氨、丙酮酸和高半胱氨酸,后者是L-甲硫氨酸的直接前体。为了更深入地了解该酶的功能和动力学性质,通过紫外可见吸收光谱、荧光光谱和圆二色光谱,在有无底物及底物类似物的情况下,对两个高度保守的活性位点残基Y55F和Y114F的突变体进行了表征,并进行了稳态动力学研究。在pH 8.5时,用苯丙氨酸取代酪氨酸55明显导致K(d)(PLP)下降130倍,这证明酪氨酸55在辅因子结合中起作用。此外,光谱数据表明该突变体积累了外部醛亚胺中间体,这表明羟基部分与PLP结合残基赖氨酸222之间缺乏相互作用导致底物去质子化速率降低。用苯丙氨酸取代酪氨酸114对L-胱硫醚的水解有轻微影响,与野生型酶相比,导致对L-丝氨酸和O-乙酰-L-丝氨酸的底物特异性发生变化。这些发现与计算数据一起,为C-S裂解酶的底物特异性提供了有用的见解,该酶的底物特异性似乎受活性位点结构和底物结合的特定构象调节,将有助于抑制剂的开发。

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