阿留申水貂病病毒在CRFK细胞中的转录谱是由单个启动子产生的前体mRNA的可变加工产生的。
The transcription profile of Aleutian mink disease virus in CRFK cells is generated by alternative processing of pre-mRNAs produced from a single promoter.
作者信息
Qiu Jianming, Cheng Fang, Burger Lisa R, Pintel David
机构信息
Department of Molecular Microbiology and Immunology, University of Missouri-Columbia, School of Medicine, Life Sciences Center, 1201 E. Rollins Rd., Columbia, MO 65211-7310, USA.
出版信息
J Virol. 2006 Jan;80(2):654-62. doi: 10.1128/JVI.80.2.654-662.2006.
Abstract
A reevaluation of the transcription profile of Aleutian mink disease parvovirus (AMDV)-infected CRFK cells at either 32 degrees C or 37 degrees C has determined that strain AMDV-G encodes six species of mRNAs produced by alternative splicing and alternative polyadenylation of a pre-mRNA generated by a single promoter at the left end of the genome. Three different splicing patterns are used, and each type is found polyadenylated at either the 3' end of the genome (the distal site) or at a site in the center of the genome (the proximal site). All spliced species accumulate similarly over the course of infection, with the R2 RNA predominant throughout. The R2 RNA, which contains and can express the NS2 coding region, encodes the viral capsid proteins VP1 and VP2.
摘要
对感染阿留申水貂病细小病毒(AMDV)的CRFK细胞在32摄氏度或37摄氏度下的转录谱进行的重新评估确定,AMDV - G毒株编码六种mRNA,这些mRNA是由基因组左端单个启动子产生的前体mRNA通过可变剪接和可变聚腺苷酸化产生的。使用了三种不同的剪接模式,并且每种类型在基因组的3'端(远端位点)或基因组中心的位点(近端位点)被聚腺苷酸化。在感染过程中,所有剪接后的种类积累情况相似,其中R2 RNA在整个过程中占主导地位。R2 RNA包含并可表达NS2编码区,编码病毒衣壳蛋白VP1和VP2。
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The transcription profile of Aleutian mink disease virus in CRFK cells is generated by alternative processing of pre-mRNAs produced from a single promoter.阿留申水貂病病毒在CRFK细胞中的转录谱是由单个启动子产生的前体mRNA的可变加工产生的。
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