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Novel insights into gene regulation of the rudivirus SIRV2 infecting Sulfolobus cells

机译:对Rudivirus SIRV2感染Sulphobus细胞的基因调控的新见解。

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Microarray analysis of infection by a lytic Sulfolobus rudivirus, SIRV2, revealed both the temporal expression of viral genes and the differential regulation of host genes. A highly susceptible strain derived from Sulfolobus solfataricus P2 with a large genomic deletion spanning CRISPR clusters A to D was infected with SIRV2, and subjected to a microarray analysis. Transcripts from a few viral genes were detected at 15 min post-infection and all except one were expressed within 2 h. The earliest expressed genes were located mainly at the termini of the linear viral genome while later expressed genes were concentrated in the central region. Timing of the expression correlated with the known or predicted functions of the viral gene products and, thus, should facilitate functional characterization of many hypothetical viral genes. Evaluation of the microarray data with quantitative reverse-transcription PCR analyses of a few selected viral genes revealed a good correlation between the two methods. Expression of about 3,000 host genes was examined. Seventy-two were downregulated > 2-fold that were mainly associated with stress response and vesicle formation, as well as chromosome structure maintenance, which appears to contribute to host chromosome degradation and cellular collapse. A further 76 host genes were upregulated > 2-fold and they were dominated by genes associated with metabolism and membrane transport, including phosphate transport and DNA precursor synthesis. The altered transcriptional patterns suggest that the virus reprograms the host cellular machinery to facilitate its own DNA replication and to inhibit cellular processes required for defense against viruses.
机译:对溶菌性硫代细小狂犬病病毒SIRV2感染进行的微阵列分析显示,病毒基因的瞬时表达和宿主基因的差异调节。用SIRV2感染了一个高度敏感的菌株,该菌株来自Sulfolobus solfataricus P2,具有跨越CRISPR簇A至D的大基因组缺失,并感染了SIRV2,并进行了微阵列分析。在感染后15分钟检测到一些病毒基因的转录本,除1个外所有基因均在2小时内表达。最早表达的基因主要位于线性病毒基因组的末端,而后来表达的基因则集中在中央区域。表达的时机与病毒基因产物的已知或预测功能有关,因此应有助于许多假想的病毒基因的功能表征。使用一些选定的病毒基因的定量逆转录PCR分析对微阵列数据进行评估,发现两种方法之间具有良好的相关性。检查了约3,000个宿主基因的表达。七十二个下调> 2倍,主要与应激反应和囊泡形成以及染色体结构维持有关,这似乎有助于宿主染色体降解和细胞崩溃。另有76个宿主基因被上调> 2倍,并以与代谢和膜运输(包括磷酸盐运输和DNA前体合成)相关的基因为主。改变的转录模式表明,病毒会对宿主细胞机制进行重新编程,以促进其自身的DNA复制并抑制防御病毒所需的细胞过程。

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