传染性胃肠炎冠状病毒包装信号位于病毒基因组的5'端。
Transmissible gastroenteritis coronavirus packaging signal is located at the 5' end of the virus genome.
作者信息
Escors David, Izeta Ander, Capiscol Carmen, Enjuanes Luis
机构信息
Department of Molecular and Cell Biology, Centro Nacional de Biotecnología, CSIC, Campus Universidad Autónoma, Cantoblanco, 28049 Madrid, Spain.
出版信息
J Virol. 2003 Jul;77(14):7890-902. doi: 10.1128/jvi.77.14.7890-7902.2003.
To locate the transmissible gastroenteritis coronavirus (TGEV) packaging signal, the incorporation of TGEV subgenomic mRNAs (sgmRNAs) into virions was first addressed. TGEV virions were purified by three different techniques, including an immunopurification using an M protein-specific monoclonal antibody. Detection of sgmRNAs in virions by specific reverse transcription-PCRs (RT-PCRs) was related to the purity of virus preparations. Interestingly, virus mRNAs were detected in partially purified virus but not in virus immunopurified using stringent conditions. Analyses by quantitative RT-PCR confirmed that virus mRNAs were not present in highly purified preparations. Lack of sgmRNA encapsidation was probably due to the absence of a packaging signal (Psi) within these mRNAs. This information plus that from the encapsidation of a collection of TGEV-derived minigenomes suggested that Psi is located at the 5' end of the genome. To confirm that this was the case, a set of minigenomes was expressed that included an expression cassette for an mRNA including the beta-glucuronidase gene (GUS) plus variable sequence fragments from the 5' end of the virus genome potentially including Psi. Insertion of the first 649 nucleotides (nt) of the TGEV genome led to the specific encapsidation of the mRNA, indicating that a Psi was located within this region which was absent from all of the other virus mRNAs. The presence of this packaging signal was further confirmed by showing the expression and rescue of the mRNA including the first 649 nt of the TGEV genome under control of the cytomegalovirus promoter in TGEV-infected cells. This mRNA was successfully amplified and encapsidated, indicating that the first 649 nt of TGEV genome also contained the 5' cis-acting replication signals. The encapsidation efficiency of this mRNA was about 30-fold higher than the genome encapsidation efficiency, as estimated by quantitative RT-PCR. In contrast, viral mRNAs presented significantly lower encapsidation efficiencies (about 100-fold) than those of the virus genome, strongly suggesting that TGEV mRNAs in fact lacked an alternative TGEV Psi.
为了定位传染性胃肠炎冠状病毒(TGEV)的包装信号,首先研究了TGEV亚基因组mRNA(sgmRNA)掺入病毒粒子的情况。通过三种不同技术纯化TGEV病毒粒子,包括使用M蛋白特异性单克隆抗体进行免疫纯化。通过特异性逆转录PCR(RT-PCR)检测病毒粒子中的sgmRNA与病毒制剂的纯度有关。有趣的是,在部分纯化的病毒中检测到病毒mRNA,但在使用严格条件免疫纯化的病毒中未检测到。定量RT-PCR分析证实,高度纯化的制剂中不存在病毒mRNA。sgmRNA未被包装可能是由于这些mRNA中不存在包装信号(Ψ)。这些信息加上来自一系列TGEV衍生的微型基因组包装的信息表明,Ψ位于基因组的5'端。为了证实情况确实如此,表达了一组微型基因组,其中包括一个用于包含β-葡萄糖醛酸酶基因(GUS)的mRNA的表达盒,以及来自病毒基因组5'端的可变序列片段,可能包括Ψ。插入TGEV基因组的前649个核苷酸(nt)导致mRNA的特异性包装,表明Ψ位于该区域内,而所有其他病毒mRNA中均不存在该区域。通过在TGEV感染的细胞中,在巨细胞病毒启动子的控制下,显示包含TGEV基因组前649 nt的mRNA的表达和拯救,进一步证实了该包装信号的存在。该mRNA成功扩增并被包装,表明TGEV基因组的前649 nt也包含5'顺式作用复制信号。通过定量RT-PCR估计,该mRNA的包装效率比基因组包装效率高约30倍。相比之下,病毒mRNA的包装效率比病毒基因组的包装效率低得多(约100倍),强烈表明TGEV mRNA实际上缺乏替代的TGEV Ψ。
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