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鉴定引物结合位点下游对于人类免疫缺陷病毒1型高效复制至关重要的序列。

Identification of sequences downstream of the primer binding site that are important for efficient replication of human immunodeficiency virus type 1.

作者信息

Li X, Liang C, Quan Y, Chandok R, Laughrea M, Parniak M A, Kleiman L, Wainberg M A

机构信息

McGill University AIDS Centre, Jewish General Hospital, and Department of Medicine, McGill University, Montreal, Quebec, Canada.

出版信息

J Virol. 1997 Aug;71(8):6003-10. doi: 10.1128/JVI.71.8.6003-6010.1997.

Abstract

Reverse transcription of retroviruses is initiated from an 18-nucleotide (nt) primer binding site (PBS), located within the 5' region of viral genomic RNA, to which the host cell-derived tRNA primer is annealed and also involves viral genomic sequences outside the PBS. We constructed proviral DNA clones of human immunodeficiency virus (HIV) that had selective deletions of either a 7-nt segment found immediately downstream of the PBS or an extended nontranslated 54-nt stretch located immediately downstream of the PBS and containing the aforementioned 7-nt segment. Synthesis of minus-strand strong-stop DNA was assessed with MT-4 cells infected with viruses derived from COS-7 cells that had been transfected with these various constructs. We found that similar levels of minus-strand strong-stop DNA as well as DNA produced after template switching were expressed in MT-4 cells infected with COS-7-derived wild-type viruses or with viruses that had the 7-nt segment deleted. In contrast, significantly lower levels of viral DNA were detected in MT-4 cells after infection with viruses that had deletions of the 54-nt stretch. Furthermore, the molecular clone containing the 7-nt deletion was able to replicate with wild-type kinetics, while that containing the 54-nt deletion displayed a significantly diminished capacity in this regard. Further deletion analysis showed that a 16-nt segment at the 3' end of this 54-nt segment was largely responsible for these effects. We also conducted studies to determine levels of viral mRNA in COS-7 cells that had been transfected with equivalent amounts of DNA derived from either a wild-type HIV construct or our various deletion mutants. In the case of transfections performed with the 7-nt deletion mutant and wild-type HIV DNA, high levels of viral mRNA transcripts were detected, which was not the case for the 54 nt-deletion mutant. However, these various mRNAs possessed similar stabilities, as shown through studies in which transcript formation was arrested by treatment of cells with actinomycin D. Thus, the 54-nt segment of 5' nontranslated RNA, located downstream of the PBS, is involved in efficient expression of each of viral DNA, mRNA, and infectious virus.

摘要

逆转录病毒的逆转录从位于病毒基因组RNA 5'区域内的一个18个核苷酸(nt)的引物结合位点(PBS)开始,宿主细胞来源的tRNA引物与该位点退火,并且还涉及PBS以外的病毒基因组序列。我们构建了人类免疫缺陷病毒(HIV)的前病毒DNA克隆,这些克隆选择性缺失了PBS下游紧邻的一个7 nt片段,或者PBS下游紧邻的一个延伸的54 nt非翻译片段,该片段包含上述7 nt片段。用MT-4细胞评估负链强终止DNA的合成,这些MT-4细胞感染了来自用这些不同构建体转染的COS-7细胞所产生的病毒。我们发现,感染COS-7来源的野生型病毒或缺失7 nt片段的病毒的MT-4细胞中,负链强终止DNA以及模板转换后产生的DNA的表达水平相似。相比之下,感染缺失54 nt片段的病毒后,MT-4细胞中检测到的病毒DNA水平显著降低。此外,含有7 nt缺失的分子克隆能够以野生型动力学进行复制,而含有54 nt缺失的克隆在这方面的能力则显著降低。进一步的缺失分析表明,这个54 nt片段3'端的一个16 nt片段在很大程度上导致了这些效应。我们还进行了研究,以确定用等量来自野生型HIV构建体或我们各种缺失突变体的DNA转染的COS-7细胞中的病毒mRNA水平。在用7 nt缺失突变体和野生型HIV DNA进行转染的情况下,检测到高水平的病毒mRNA转录本,而54 nt缺失突变体则不然。然而,通过用放线菌素D处理细胞使转录形成停止的研究表明,这些不同的mRNA具有相似的稳定性。因此,位于PBS下游的5'非翻译RNA的54 nt片段参与了病毒DNA、mRNA和感染性病毒各自的有效表达。

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本文引用的文献

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