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苜蓿银纹夜蛾多粒包埋核型多角体病毒基因在哺乳动物细胞中的表达及宿主β-肌动蛋白基因的上调

Expression of Autographa californica multiple nucleopolyhedrovirus genes in mammalian cells and upregulation of the host beta-actin gene.

作者信息

Fujita Ryosuke, Matsuyama Takahiro, Yamagishi Junya, Sahara Ken, Asano Shinichiro, Bando Hisanori

机构信息

Laboratory of Applied Molecular Entomology, Division of Applied Bioscience, Graduate School of Agriculture, Hokkaido University, Sapporo, Japan.

出版信息

J Virol. 2006 Mar;80(5):2390-5. doi: 10.1128/JVI.80.5.2390-2395.2006.

Abstract

The gene expression of Autographa californica multiple nucleopolyhedrovirus (AcMNPV) was examined in two types of mammalian cells, human HeLa14 and hamster BHK cells. DNA microarray analysis followed by reverse transcription-PCR identified at least 12 viral genes transcribed in both HeLa14 cells and BHK cells inoculated with AcMNPV. 5' rapid amplification of cDNA ends was carried out to examine the transcriptional fidelity of these genes in HeLa14 cells. The transcription of ie-1, ie-0 and gp64 was initiated at a baculovirus early gene motif, CAGT, accompanied by a TATA motif. In addition, the same splicing observed for ie-0 mRNA in Sf9 cells occurred in HeLa14 cells. While the transcription initiation sites for pe38 and p6.9 were not located in the CAGT motif, most of them were in a typical eukaryotic RNA polymerase II promoter structure (a conventional TATA motif and/or an initiator). Interestingly, the expression of beta-actin was upregulated in the mammalian cells inoculated with AcMNPV. Subsequent experiments using UV-inactivated virus confirmed the upregulation, suggesting that de novo synthesis of viral products is not required for the event. These results indicated that the AcMNPV genome acts as a template for transcription in mammalian cells through the usual infection pathway, though there is no evidence for the functional expression of viral genes at present.

摘要

在两种哺乳动物细胞,即人源HeLa14细胞和仓鼠BHK细胞中检测了苜蓿银纹夜蛾多粒包埋核型多角体病毒(AcMNPV)的基因表达。通过DNA微阵列分析并结合逆转录PCR,鉴定出在接种AcMNPV的HeLa14细胞和BHK细胞中至少有12个病毒基因被转录。进行5' cDNA末端快速扩增以检测这些基因在HeLa14细胞中的转录保真度。ie-1、ie-0和gp64的转录起始于杆状病毒早期基因基序CAGT,并伴有TATA基序。此外,在Sf9细胞中观察到的ie-0 mRNA的相同剪接也发生在HeLa14细胞中。虽然pe38和p6.9的转录起始位点不在CAGT基序中,但它们大多数位于典型的真核RNA聚合酶II启动子结构(传统的TATA基序和/或起始子)中。有趣的是,接种AcMNPV的哺乳动物细胞中β-肌动蛋白的表达上调。随后使用紫外线灭活病毒进行的实验证实了这种上调,这表明该事件不需要病毒产物的从头合成。这些结果表明,AcMNPV基因组通过通常的感染途径在哺乳动物细胞中作为转录模板,尽管目前没有证据表明病毒基因有功能性表达。

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