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一种基因7和11发生重排的人轮状病毒编码一种修饰的NSP3蛋白,并提示了基因重排的另一种机制。

A human rotavirus with rearranged genes 7 and 11 encodes a modified NSP3 protein and suggests an additional mechanism for gene rearrangement.

作者信息

Gault E, Schnepf N, Poncet D, Servant A, Teran S, Garbarg-Chenon A

机构信息

Laboratoire de Virologie, Hôpital Armand Trousseau (EA 2391, UFR Saint-Antoine), Paris, France.

出版信息

J Virol. 2001 Aug;75(16):7305-14. doi: 10.1128/JVI.75.16.7305-7314.2001.

Abstract

A human rotavirus (isolate M) with an atypical electropherotype with 14 apparent bands of double-stranded RNA was isolated from a chronically infected immunodeficient child. MA-104 cell culture adaptation showed that the M isolate was a mixture of viruses containing standard genes (M0) or rearranged genes: M1 (containing a rearranged gene 7) and M2 (containing rearranged genes 7 and 11). The rearranged gene 7 of virus M1 (gene 7R) was very unusual because it contained two complete open reading frames (ORF). Moreover, serial propagation of virus M1 in cell culture indicated that gene 7R rapidly evolved, leading to a virus with a deleted gene 7R (gene 7RDelta). Gene 7RDelta coded for a modified NSP3 protein (NSP3m) of 599 amino acids (aa) containing a repetition of aa 8 to 296. The virus M3 (containing gene 7RDelta) was not defective in cell culture and actually produced NSP3m. The rearranged gene 11 (gene 11R) had a more usual pattern, with a partial duplication leading to a normal ORF followed by a long 3' untranslated region. The rearrangement in gene 11R was almost identical to some of those previously described, suggesting that there is a hot spot for gene rearrangements at a specific location on the sequence. It has been suggested that in some cases the existence of short direct repeats could favor the occurrence of rearrangement at a specific site. The computer modeling of gene 7 and 11 mRNAs led us to propose a new mechanism for gene rearrangements in which secondary structures, besides short direct repeats, might facilitate and direct the transfer of the RNA polymerase from the 5' to the 3' end of the plus-strand RNA template during the replication step.

摘要

从一名慢性感染的免疫缺陷儿童中分离出一株具有非典型电泳图谱的人轮状病毒(分离株M),其双链RNA有14条明显条带。MA-104细胞培养适应性研究表明,M分离株是一种病毒混合物,包含标准基因(M0)或重排基因:M1(包含重排的基因7)和M2(包含重排的基因7和11)。病毒M1的重排基因7(基因7R)非常特殊,因为它包含两个完整的开放阅读框(ORF)。此外,病毒M1在细胞培养中的连续传代表明基因7R迅速进化,产生了一个缺失基因7R的病毒(基因7RDelta)。基因7RDelta编码一种599个氨基酸(aa)的修饰NSP3蛋白(NSP3m),其中包含aa 8至296的重复序列。病毒M3(包含基因7RDelta)在细胞培养中没有缺陷,实际上产生了NSP3m。重排基因11(基因11R)具有更常见的模式,部分重复导致一个正常的ORF,随后是一个长的3'非翻译区。基因11R中的重排与先前描述的一些重排几乎相同,表明在序列的特定位置存在基因重排热点。有人提出,在某些情况下,短直接重复序列的存在可能有利于特定位点重排的发生。基因7和11 mRNA的计算机建模使我们提出了一种新的基因重排机制,其中除了短直接重复序列外,二级结构可能在复制步骤中促进并指导RNA聚合酶从正链RNA模板的5'端转移到3'端。

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