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DNA结合提供了一条激活腺病毒蛋白酶的分子带。

DNA binding provides a molecular strap activating the adenovirus proteinase.

作者信息

Gupta Sayan, Mangel Walter F, McGrath William J, Perek Jennifer L, Lee Donna W, Takamoto Keiji, Chance Mark R

机构信息

Center for Synchrotron Biosciences, Department of Physiology & Biophysics, Albert Einstein College of Medicine, Bronx, NY 10461, USA

出版信息

Mol Cell Proteomics. 2004 Oct;3(10):950-9. doi: 10.1074/mcp.M400037-MCP200. Epub 2004 Jun 24.

Abstract

Human adenovirus proteinase (AVP) requires two cofactors for maximal activity: pVIc, a peptide derived from the C terminus of adenovirus precursor protein pVI, and the viral DNA. Synchrotron protein footprinting was used to map the solvent accessible cofactor binding sites and to identify conformational changes associated with the binding of cofactors to AVP. The binding of pVIc alone or pVIc and DNA together to AVP triggered significant conformational changes adjacent to the active site cleft sandwiched between the two AVP subdomains. In addition, upon binding of DNA to AVP, it was observed that specific residues on each of the two major subdomains were significantly protected from hydroxyl radicals. Based on the locations of these protected side-chain residues and conserved aromatic and positively charged residues within AVP, a three-dimensional model of DNA binding was constructed. The model indicated that DNA binding can alter the relative orientation of the two AVP domains leading to the partial activation of AVP by DNA. In addition, both pVIc and DNA may independently alter the active site conformation as well as drive it cooperatively to fully activate AVP.

摘要

人腺病毒蛋白酶(AVP)需要两种辅助因子才能达到最大活性:pVIc,一种源自腺病毒前体蛋白pVI C末端的肽,以及病毒DNA。同步加速器蛋白质足迹法用于绘制溶剂可及的辅助因子结合位点,并确定与辅助因子与AVP结合相关的构象变化。单独的pVIc或pVIc与DNA一起与AVP结合会引发两个AVP亚结构域之间活性位点裂隙附近的显著构象变化。此外,在DNA与AVP结合后,观察到两个主要亚结构域上的特定残基受到显著的羟基自由基保护。基于这些受保护侧链残基的位置以及AVP内保守的芳香族和带正电荷的残基,构建了DNA结合的三维模型。该模型表明,DNA结合可改变两个AVP结构域的相对取向,导致DNA对AVP的部分激活。此外,pVIc和DNA均可独立改变活性位点构象,并协同驱动其完全激活AVP。

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