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莫氏异蚤蝇昆虫痘病毒的球形体蛋白基因在脊椎动物痘病毒中转录错误。

The Amsacta moorei entomopoxvirus spheroidin gene is improperly transcribed in vertebrate poxviruses.

作者信息

Hall R L, Li Y, Feller J, Moyer R W

机构信息

Department of Molecular Genetics and Microbiology; College of Medicine, University of Florida, Gainesville 32610-0266, USA.

出版信息

Virology. 1996 Oct 15;224(2):427-36. doi: 10.1006/viro.1996.0549.

Abstract

The Amsacta moorei entomopoxvirus (AmEPv) spheroidin is the most highly expressed late viral gene product in infected insect cells. However, when a cassette containing the spheroidin gene and putative promoter was inserted into cowpox (CPV) or vaccinia viruses, only very low levels of spheroldin gene expression were observed. Primer extension analysis suggests much lower spheroidin gene transcript levels than seen either for the highly expressed CPV A-type inclusion gene or for the spheroidin gene within infected insect cells, indicating that in vertebrate cells, the spheroidin promoter functions poorly if at all. Examination of the spheroidin mRNA synthesized in recombinant CPV shows that the 5' start site of the spheroidin transcript was also unexpectedly imprecise and upstream (approximately 31 bp) of the well-defined start site normally observed in AmEPV-infected insect cells. Sequencing of the 5' terminus of the CPV recombinant spheroidin mRNA suggested that 5' poly(A), a characteristic feature of late poxvirus mRNAs and spheroidin mRNA derived from insect cells, was absent, despite the presence of the typical vertebrate poxvirus late promoter consensus sequence, TAAATG. Our results indicate that insect and vertebrate poxvirus promoters may not be universally interchangeable and imply that there are regulatory features of gene expression unique to the infected insect cell environment.

摘要

莫氏异跗萤叶甲昆虫痘病毒(AmEPv)的球形体蛋白是感染昆虫细胞中表达量最高的晚期病毒基因产物。然而,当将一个包含球形体蛋白基因和推定启动子的盒式结构插入牛痘病毒(CPV)或痘苗病毒时,仅观察到极低水平的球形体蛋白基因表达。引物延伸分析表明,球形体蛋白基因转录水平比高表达的CPV A型包涵体基因或感染昆虫细胞中的球形体蛋白基因的转录水平低得多,这表明在脊椎动物细胞中,球形体蛋白启动子即使有功能也很差。对重组CPV中合成的球形体蛋白mRNA的检查表明,球形体蛋白转录本的5'起始位点也出人意料地不精确,且位于AmEPv感染的昆虫细胞中通常观察到的明确起始位点的上游(约31 bp)。对CPV重组球形体蛋白mRNA的5'末端进行测序表明,尽管存在典型的脊椎动物痘病毒晚期启动子共有序列TAAATG,但源自昆虫细胞的晚期痘病毒mRNA和球形体蛋白mRNA的特征性5'多聚腺苷酸(poly(A))却不存在。我们的结果表明,昆虫痘病毒和脊椎动物痘病毒的启动子可能并非普遍可互换,这意味着在感染昆虫细胞的环境中存在基因表达的独特调控特征。

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