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风疹病毒假定复制酶的视网膜母细胞瘤蛋白结合LXCXE基序中的突变影响病毒复制。

Mutations in the retinoblastoma protein-binding LXCXE motif of rubella virus putative replicase affect virus replication.

作者信息

Forng R Y, Atreya C D

出版信息

J Gen Virol. 1999 Feb;80 ( Pt 2):327-332. doi: 10.1099/0022-1317-80-2-327.

DOI:10.1099/0022-1317-80-2-327
PMID:10073691
Abstract

The rubella virus (RV)-encoded protein NSP90, which contains the retinoblastoma protein (Rb)-binding motif LXCXE, interacts with Rb and RV replication is reduced in cells lacking Rb. Whether the LXCXE motif of RV NSP90 itself is essential for Rb binding and virus replication is not known. Therefore, in the present study, the functional role of this motif was investigated by site-directed mutagenesis in a plasmid from which infectious RV RNA can be produced. Three critical mutations in the motif, two substitutions at the conserved cysteine residue (C --> G and C --> R) and a deletion of the entire motif, were created. A cell-free translated NSP90 C terminus polypeptide containing the deletion did not bind to Rb and a polypeptide carrying the C --> R substitution had barely detectable binding affinity for Rb. Rb binding by the C --> G mutant was reduced significantly compared to that of wild-type protein. Correlating with the binding results, mutant viruses containing the LXRXE and LXGXE motifs had a reduction in replication to < 0.5% and 47% of the wild-type, respectively, while deletion of the motif was found to be lethal. By the first serial passage, replication of the LXRXE-carrying virus had increased from < 0.5% to 2% of the wild-type. Sequencing of the genome of this virus revealed a nucleotide change that altered the motif from LXRXE to LXSXE, which is a known Rb-binding motif in two protein phosphatase subunits. Thus, our results clearly demonstrate that the LXCXE motif is required for efficient RV replication.

摘要

风疹病毒(RV)编码的蛋白NSP90含有视网膜母细胞瘤蛋白(Rb)结合基序LXCXE,它与Rb相互作用,并且在缺乏Rb的细胞中RV复制减少。RV NSP90自身的LXCXE基序对于Rb结合和病毒复制是否至关重要尚不清楚。因此,在本研究中,通过定点诱变在一个可产生传染性RV RNA的质粒中研究了该基序的功能作用。在该基序中产生了三个关键突变,即保守半胱氨酸残基的两个替换(C→G和C→R)以及整个基序的缺失。一个含有缺失的无细胞翻译的NSP90 C末端多肽不与Rb结合,而携带C→R替换的多肽对Rb的结合亲和力几乎检测不到。与野生型蛋白相比,C→G突变体与Rb的结合显著减少。与结合结果相关的是,含有LXRXE和LXGXE基序的突变病毒的复制分别降至野生型的<0.5%和47%,而发现基序缺失是致死性的。在第一次连续传代时,携带LXRXE的病毒的复制从<0.5%增加到野生型的2%。对该病毒基因组的测序揭示了一个核苷酸变化,该变化将基序从LXRXE改变为LXSXE,这是两个蛋白磷酸酶亚基中已知的Rb结合基序。因此,我们的结果清楚地表明LXCXE基序是RV高效复制所必需的。

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