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通过光亲和标记和质谱法对人乳头瘤病毒11型E1-E2蛋白相互作用抑制剂在E2反式激活结构域上的结合位点进行表征。

Characterization of the binding site for inhibitors of the HPV11 E1-E2 protein interaction on the E2 transactivation domain by photoaffinity labeling and mass spectrometry.

作者信息

Davidson Walter, McGibbon Graham A, White Peter W, Yoakim Christiane, Hopkins Jerry L, Guse Ingrid, Hambly David M, Frego Lee, Ogilvie William W, Lavallée Pierre, Archambault Jacques

机构信息

Research and Development, Boehringer Ingelheim (Canada) Ltd., 2100 Cunard Street, Laval, Québec, Canada H7S 2G5.

出版信息

Anal Chem. 2004 Apr 1;76(7):2095-102. doi: 10.1021/ac035335o.

DOI:10.1021/ac035335o
PMID:15053675
Abstract

An indandione-containing class of inhibitors abrogates DNA replication of human papillomavirus (HPV) types 6 and 11 by binding reversibly to the transactivation domain (TAD) of the viral E2 protein and inhibiting its interaction with the viral E1 helicase. To locate the binding site of this class of protein-protein interaction inhibitors, a benzophenone derivative was used to generate an irreversibly labeled E2-TAD polypeptide. The single site of covalent modification of the E2-TAD was identified by proteolytic digestions using trypsin, LysC, and V8 proteases and characterization of the resulting peptides by LC-MS procedures. Through this methodology, the benzophenone attachment point was located at the terminal methyl of residue Met101. Evidence further pinpointed the site of photoaffinity attachment to the terminal carbon atom, which is significant in providing a definitive example of the ability to locate photoinduced cross-linking to a polypeptide with atomic resolution using solely mass spectrometric detection. The location of the inhibitor binding site vis-à-vis the Glu39 and Glu100 residues sensitive to mutation for HPV 11 E2-TAD is discussed in relation to the crystal structure of the E2-TAD from the related HPV type 16.

摘要

一类含茚二酮的抑制剂通过与病毒E2蛋白的反式激活结构域(TAD)可逆结合并抑制其与病毒E1解旋酶的相互作用,从而废除人乳头瘤病毒(HPV)6型和11型的DNA复制。为了定位这类蛋白质-蛋白质相互作用抑制剂的结合位点,使用一种二苯甲酮衍生物生成了一种不可逆标记的E2-TAD多肽。通过使用胰蛋白酶、LysC和V8蛋白酶进行蛋白水解消化,并通过液相色谱-质谱法(LC-MS)对所得肽段进行表征,确定了E2-TAD的共价修饰单一位点。通过这种方法,二苯甲酮连接点位于残基Met101的末端甲基处。证据进一步确定了光亲和连接位点为末端碳原子,这对于仅使用质谱检测以原子分辨率定位光诱导交联到多肽的能力提供了一个明确的例子具有重要意义。结合来自相关HPV 16型的E2-TAD的晶体结构,讨论了抑制剂结合位点相对于对HPV 11 E2-TAD突变敏感的Glu39和Glu100残基的位置。

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Characterization of the binding site for inhibitors of the HPV11 E1-E2 protein interaction on the E2 transactivation domain by photoaffinity labeling and mass spectrometry.通过光亲和标记和质谱法对人乳头瘤病毒11型E1-E2蛋白相互作用抑制剂在E2反式激活结构域上的结合位点进行表征。
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