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人Hyal1的透明质酸酶活性需要活性位点的酸性和酪氨酸残基。

Hyaluronidase activity of human Hyal1 requires active site acidic and tyrosine residues.

作者信息

Zhang Ling, Bharadwaj Alamelu G, Casper Andrew, Barkley Joel, Barycki Joseph J, Simpson Melanie A

机构信息

Department of Biochemistry, University of Nebraska, Lincoln, Nebraska 68588-0664, USA.

出版信息

J Biol Chem. 2009 Apr 3;284(14):9433-42. doi: 10.1074/jbc.M900210200. Epub 2009 Feb 6.

DOI:10.1074/jbc.M900210200
PMID:19201751
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2666596/
Abstract

Hyaluronidases are a family of endolytic glycoside hydrolases that cleave the beta1-4 linkage between N-acetylglucosamine and glucuronic acid in hyaluronan polymers via a substrate-assisted mechanism. In humans, turnover of hyaluronan by this enzyme family is critical for normal extracellular matrix remodeling. However, elevated expression of the Hyal1 isozyme accelerates tumor growth and metastatic progression. In this study, we used structural information, site-directed mutagenesis, and steady state enzyme kinetics to probe molecular determinants of human Hyal1 function. Mutagenesis of active site residues Glu(131) and Tyr(247) to Gln and Phe, respectively, eliminated activity at all hyaluronan concentrations (to 125 microm or 2.5 mg/ml). Conservative mutagenesis of Asp(129) and Tyr(202) significantly impaired catalysis by increases of 5- and 10-fold in apparent K(m) and reductions in V(max) of 95 and 50%, respectively. Tyr(247) and Asp(129) are required for stabilization of the catalytic nucleophile, which arises as a resonance intermediate of N-acetylglucosamine on the substrate. Glu(131) is a likely proton donor for the hydroxyl leaving group. Tyr(202) is a substrate binding determinant. General disulfide reduction had no effect on activity in solution, but enzymatic deglycosylation reduced Hyal1 activity in a time-dependent fashion. Mutagenesis identified Asn(350) glycosylation as the requisite modification. Deletion of the C-terminal epidermal growth factor-like domain, in which Asn(350) is located, also eliminated activity, irrespective of glycosylation. Collectively, these studies define key components of Hyal1 active site catalysis, and structural factors critical for stability. Such detailed understanding will allow rational design of enzyme modulators.

摘要

透明质酸酶是一类内切糖苷水解酶,通过底物辅助机制切割透明质酸聚合物中N - 乙酰葡糖胺和葡糖醛酸之间的β1-4键。在人类中,该酶家族对透明质酸的周转对于正常的细胞外基质重塑至关重要。然而,Hyal1同工酶的表达升高会加速肿瘤生长和转移进程。在本研究中,我们利用结构信息、定点诱变和稳态酶动力学来探究人类Hyal1功能的分子决定因素。分别将活性位点残基Glu(131)和Tyr(247)突变为Gln和Phe,在所有透明质酸浓度下(至125微摩尔或2.5毫克/毫升)均消除了活性。Asp(129)和Tyr(202)的保守诱变显著损害了催化作用,表观K(m)分别增加了5倍和10倍,V(max)分别降低了95%和50%。Tyr(247)和Asp(129)是稳定催化亲核试剂所必需的,该亲核试剂是底物上N - 乙酰葡糖胺的共振中间体。Glu(131)可能是羟基离去基团的质子供体。Tyr(202)是底物结合决定因素。一般的二硫键还原对溶液中的活性没有影响,但酶促去糖基化以时间依赖性方式降低了Hyal1活性。诱变确定Asn(350)糖基化是必需的修饰。缺失Asn(350)所在的C末端表皮生长因子样结构域也消除了活性,无论糖基化情况如何。总体而言,这些研究确定了Hyal1活性位点催化作用的关键成分以及对稳定性至关重要的结构因素。这种详细的理解将有助于合理设计酶调节剂。

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