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本文引用的文献

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Genomic analysis of diverse rubella virus genotypes.不同风疹病毒基因型的基因组分析
J Gen Virol. 2007 Mar;88(Pt 3):932-941. doi: 10.1099/vir.0.82495-0.
2
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Proteins. 2006 Nov 15;65(3):643-55. doi: 10.1002/prot.21139.
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Using protein design to dissect the effect of charged residues on metal binding and protein stability.利用蛋白质设计剖析带电荷残基对金属结合及蛋白质稳定性的影响。
Biochemistry. 2006 May 9;45(18):5848-56. doi: 10.1021/bi052508q.
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Predicting calcium-binding sites in proteins - a graph theory and geometry approach.预测蛋白质中的钙结合位点——一种图论与几何学方法。
Proteins. 2006 Jul 1;64(1):34-42. doi: 10.1002/prot.20973.
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Analysis of rubella virus capsid protein-mediated enhancement of replicon replication and mutant rescue.风疹病毒衣壳蛋白介导的复制子复制增强及突变体拯救分析
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Virus factories: associations of cell organelles for viral replication and morphogenesis.病毒工厂:用于病毒复制和形态发生的细胞器关联
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DICHROWEB, an online server for protein secondary structure analyses from circular dichroism spectroscopic data.DICHROWEB,一个用于从圆二色光谱数据进行蛋白质二级结构分析的在线服务器。
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风疹病毒非结构蛋白酶中钙离子结合结构域的鉴定

Identification of a Ca2+-binding domain in the rubella virus nonstructural protease.

作者信息

Zhou Yubin, Tzeng Wen-Pin, Yang Wei, Zhou Yumei, Ye Yiming, Lee Hsiau-wei, Frey Teryl K, Yang Jenny

机构信息

Department of Chemistry, Georgia State University, 50 Decatur St., Atlanta, GA 30303, USA.

出版信息

J Virol. 2007 Jul;81(14):7517-28. doi: 10.1128/JVI.00605-07. Epub 2007 May 2.

DOI:10.1128/JVI.00605-07
PMID:17475644
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1933374/
Abstract

The rubella virus (RUB) nonstructural protein (NS) open reading frame (ORF) encodes a polypeptide precursor that is proteolytically self cleaved into two replicase components involved in viral RNA replication. A putative EF-hand Ca(2+)-binding motif that was conserved across different genotypes of RUB was predicted within the nonstructural protease that cleaves the precursor by using bioinformatics tools. To probe the metal-binding properties of this motif, we used an established grafting approach and engineered the 12-residue Ca(2+)-coordinating loop into a non-Ca(2+)-binding scaffold protein, CD2. The grafted EF-loop bound to Ca(2+) and its trivalent analogs Tb(3+) and La(3+) with K(d)s of 214, 47, and 14 microM, respectively. Mutations (D1210A and D1217A) of two of the potential Ca(2+)-coordinating ligands in the EF-loop led to the elimination of Tb(3+) binding. Inductive coupled plasma mass spectrometry was used to confirm the presence of Ca(2+) ([Ca(2+)]/[protein] = 0.7 +/- 0.2) in an NS protease minimal metal-binding domain, RUBCa, that spans the EF-hand motif. Conformational studies on RUBCa revealed that Ca(2+) binding induced local conformational changes and increased thermal stability (Delta T(m) = 4.1 degrees C). The infectivity of an RUB infectious cDNA clone containing the mutations D1210A/D1217A was decreased by approximately 20-fold in comparison to the wild-type (wt) clone, and these mutations rapidly reverted to the wt sequence. The NS protease containing these mutations was less efficient at precursor cleavage than the wt NS protease at 35 degrees C, and the mutant NS protease was temperature sensitive at 39 degrees C, confirming that the Ca(2+)-binding loop played a structural role in the NS protease and was specifically required for optimal stability under physiological conditions.

摘要

风疹病毒(RUB)非结构蛋白(NS)开放阅读框(ORF)编码一种多肽前体,该前体经蛋白水解后自我切割成两个参与病毒RNA复制的复制酶成分。利用生物信息学工具,在切割前体的非结构蛋白酶中预测到一个假定的EF手型Ca(2+)结合基序,该基序在不同基因型的RUB中保守。为了探究该基序的金属结合特性,我们采用了一种既定的嫁接方法,将12个残基的Ca(2+)配位环工程化到一种非Ca(2+)结合支架蛋白CD2中。嫁接的EF环与Ca(2+)及其三价类似物Tb(3+)和La(3+)结合,解离常数(K(d))分别为214、47和14微摩尔。EF环中两个潜在的Ca(2+)配位配体的突变(D1210A和D1217A)导致Tb(3+)结合的消除。电感耦合等离子体质谱法用于确认在跨越EF手型基序的NS蛋白酶最小金属结合结构域RUBCa中存在Ca(2+)([Ca(2+)]/[蛋白]=0.7±0.2)。对RUBCa的构象研究表明,Ca(2+)结合诱导局部构象变化并增加热稳定性(ΔT(m)=4.1℃)。与野生型(wt)克隆相比,含有D1210A/D1217A突变的RUB感染性cDNA克隆的感染性降低了约20倍,并且这些突变迅速回复到wt序列。含有这些突变的NS蛋白酶在35℃时对前体切割的效率低于wt NS蛋白酶,并且突变型NS蛋白酶在39℃时对温度敏感,证实Ca(2+)结合环在NS蛋白酶中起结构作用,并且在生理条件下对最佳稳定性是特异性必需的。