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禽成髓细胞瘤病毒转化基因与其辅助病毒之间的重组位点。

Sites of recombination between the transforming gene of avian myeloblastosis virus and its helper virus.

作者信息

Kan N C, Baluda M A, Papas T S

出版信息

Virology. 1985 Sep;145(2):323-9. doi: 10.1016/0042-6822(85)90166-7.

Abstract

The sites of recombination between the transforming gene of avian myeloblastosis virus (AMV) and its natural helper myeloblastosis-associated virus (MAV) have been determined. In AMV, the cellular sequence substituting for the viral envelope (env) gene gives rise to a different carboxyl terminus of the DNA polymerase. The 5'-recombination site coincides with the RNA splice acceptor site for the production of env mRNA in MAV-infected cells. The 3'-recombination site reveals that the last 11 amino acids including the termination codon are shared by the env protein and AMV transforming protein. The RNA splice acceptor site for the generation of subgenomic v-myb mRNA is located 84 nucleotides downstream from the 5'-recombination site. The AMV transforming protein consists of helper virus-related sequences at both of its amino and carboxyl termini, and all but 84 nucleotides of the cell-derived v-myb sequence. The comparison of MAV gp85 amino acid sequence with those of subgroups B, C, and E indicates that the MAV present in clone lambda 10A2-1 belongs to subgroup B. The high degree of homology among different avian retroviruses of the same subgroup indicates that the amino acid sequence of gp85 is important in determining the conformation of the envelope glycoprotein.

摘要

已确定禽成髓细胞瘤病毒(AMV)的转化基因与其天然辅助成髓细胞瘤相关病毒(MAV)之间的重组位点。在AMV中,取代病毒包膜(env)基因的细胞序列会产生不同的DNA聚合酶羧基末端。5'重组位点与MAV感染细胞中产生env mRNA的RNA剪接受体位点重合。3'重组位点表明,包括终止密码子在内的最后11个氨基酸由env蛋白和AMV转化蛋白共享。产生亚基因组v-myb mRNA的RNA剪接受体位点位于5'重组位点下游84个核苷酸处。AMV转化蛋白在其氨基末端和羧基末端均由与辅助病毒相关的序列组成,并且除了84个核苷酸外,均为细胞来源的v-myb序列。将MAV gp85氨基酸序列与B、C和E亚组的序列进行比较表明,克隆λ10A2-1中存在的MAV属于B亚组。同一亚组的不同禽逆转录病毒之间的高度同源性表明,gp85的氨基酸序列在确定包膜糖蛋白的构象中很重要。

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