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MutY 同源物(MYH)的分离与分析。

Isolation and analyses of MutY homologs (MYH).

作者信息

Lu-Chang A-Lien

机构信息

University of Maryland, Department of Biochemistry, Baltimore, USA.

出版信息

Methods Enzymol. 2006;408:64-78. doi: 10.1016/S0076-6879(06)08005-0.

DOI:10.1016/S0076-6879(06)08005-0
PMID:16793363
Abstract

The base excision repair carried out by the bacterial MutY DNA glycosylase and eukaryotic MutY homolog (MYH) is responsible for removing adenines misincorporated into DNA opposite 7,8-dihydro-8-oxo-guanines (8-oxoG), thereby preventing G:C to T:A mutations. MutY and MYH can also remove adenines from A/G and A/C and can remove guanines from G/8-oxoG mismatches at reduced rates. Biallelic germline mutations in the human MYH gene predispose individuals to multiple colorectal adenomas and carcinoma. Four functional assays are usually employed to characterize the MutY and MYH. Gel mobility shift or fluorescence anisotropy assays measures DNA-binding affinity and the apparent dissociation constants. Glycosylase assay determines the catalytic parameters of the enzyme. By using a trapping assay in the presence of sodium borohydride, the protein-DNA covalent intermediate can be identified. The in vivo activity of MutY or MYH can be measured by complementation in Escherichia coli mutY mutants or fission yeast Schizosaccharomyces pombe MYH knockout cells. MutY and MYH interacting proteins can be analyzed by the glutathione S-transferase pull-down assay, Far-western, and coimmunoprecipitation. The in vitro and in vivo activities of MYH can be modulated by several proteins, including mismatch recognition enzymes MSH2/MSH6, proliferating cell nuclear antigen, and apurinic/apyrimidinic endonuclease.

摘要

由细菌MutY DNA糖基化酶和真核MutY同源物(MYH)进行的碱基切除修复负责去除错配掺入到与7,8-二氢-8-氧代鸟嘌呤(8-氧代G)相对的DNA中的腺嘌呤,从而防止G:C到T:A的突变。MutY和MYH还可以从A/G和A/C中去除腺嘌呤,并且可以以较低的速率从G/8-氧代G错配中去除鸟嘌呤。人类MYH基因的双等位基因种系突变使个体易患多发性结肠直肠腺瘤和癌。通常采用四种功能测定来表征MutY和MYH。凝胶迁移率变动分析或荧光偏振分析测量DNA结合亲和力和表观解离常数。糖基化酶分析确定酶的催化参数。通过在硼氢化钠存在下使用捕获分析,可以鉴定蛋白质-DNA共价中间体。MutY或MYH的体内活性可以通过在大肠杆菌mutY突变体或裂殖酵母粟酒裂殖酵母MYH敲除细胞中的互补来测量。MutY和MYH相互作用蛋白可以通过谷胱甘肽S-转移酶下拉分析、Far-western和免疫共沉淀进行分析。MYH的体外和体内活性可以被几种蛋白质调节,包括错配识别酶MSH2/MSH6、增殖细胞核抗原和脱嘌呤/脱嘧啶内切核酸酶。

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