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影响v-Abl蛋白MA部分的突变揭示了Gag在艾贝尔逊鼠白血病病毒(MLV)和莫洛尼MLV中的保守作用。

Mutations affecting the MA portion of the v-Abl protein reveal a conserved role of Gag in Abelson murine leukemia virus (MLV) and Moloney MLV.

作者信息

Yi Chae-ryun, Rosenberg Naomi

机构信息

Molecular Microbiology Graduate Program, Sackler School of Graduate Biomedical Sciences, Boston, Massachusetts 02111, USA.

出版信息

J Virol. 2008 Jun;82(11):5307-15. doi: 10.1128/JVI.00089-08. Epub 2008 Mar 26.

Abstract

Abelson murine leukemia virus (Ab-MLV) arose from a recombination between gag sequences in Moloney MLV (Mo-MLV) and the c-abl proto-oncogene. The v-Abl oncoprotein encoded by Ab-MLV contains MA, p12, and a portion of CA sequences derived from the gag gene of Mo-MLV. Previous studies indicated that alteration of MA sequences affects the biology of Mo-MLV and Ab-MLV. To understand the role of these sequences in Ab-MLV transformation more fully, alanine substitution mutants that affect Mo-MLV replication were examined in the context of Ab-MLV. Mutations affecting Mo-MLV replication decreased transformation, while alanine mutations in residues dispensable for Mo-MLV replication did not. The altered v-Abl proteins displayed aberrant subcellular localization that correlated to transformation defects. Immunofluorescent analyses suggested that aberrant trafficking of the altered proteins and improper interaction with components of the cytoskeleton were involved in the phenotype. Similar defects in localization were observed when the Gag moiety containing these mutations was expressed in the absence of abl-derived sequences. These results indicate that MA sequences within the Gag moiety of the v-Abl protein contribute to proper localization by playing a dominant role in trafficking of the v-Abl molecule.

摘要

阿贝尔逊鼠白血病病毒(Ab-MLV)源于莫洛尼鼠白血病病毒(Mo-MLV)的gag序列与c-abl原癌基因之间的重组。由Ab-MLV编码的v-Abl癌蛋白包含源自Mo-MLV gag基因的MA、p12和部分CA序列。先前的研究表明,MA序列的改变会影响Mo-MLV和Ab-MLV的生物学特性。为了更全面地了解这些序列在Ab-MLV转化中的作用,在Ab-MLV背景下检测了影响Mo-MLV复制的丙氨酸替代突变体。影响Mo-MLV复制的突变会降低转化效率,而对Mo-MLV复制可有可无的残基中的丙氨酸突变则不会。改变后的v-Abl蛋白表现出异常的亚细胞定位,这与转化缺陷相关。免疫荧光分析表明,改变后的蛋白的异常运输以及与细胞骨架成分的不适当相互作用参与了该表型。当在没有abl衍生序列的情况下表达含有这些突变的Gag部分时,观察到类似的定位缺陷。这些结果表明,v-Abl蛋白的Gag部分内的MA序列通过在v-Abl分子的运输中起主导作用,有助于正确定位。

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