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FBR-骨肉瘤病毒复合体的基因组组织:亚基因组fos特异性信息的鉴定。

Genome organisation of the FBR-osteosarcoma virus complex: identification of a subgenomic fos-specific message.

作者信息

Michiels L, van Roy F, de Saint-Georges L, Merregaert J

出版信息

Virus Res. 1986 Jul;5(1):11-26. doi: 10.1016/0168-1702(86)90062-6.

Abstract

The FBR murine virus complex together with the FBJ murine virus complex are known to be bone tumor inducers in newborn mice. Both transforming viruses have transduced c-proto-fos-derived sequences in their genome. FBR-MuSV was molecularly cloned as a biologically active 10-kbp EcoRI fragment from non-productively transformed rat embryo fibroblasts into Charon phage 4A (lambda MOL503) and subsequently subcloned in plasmid pBR322 (pMOL503). Its natural associated helper FBR-MuLV, excized as an internal 8.2-kbp PstI proviral DNA fragment from chronically infected NIH/3T3 cells, was cloned into the unique PstI site of pBR322. Comparative analysis of the restriction maps of FBR-MuSV and FBR-MuLV together with the electron microscopic analysis of heteroduplex DNA molecules formed between both molecular clones suggested that FBR-MuLV is the parental virus of FBR-MuSV. fos- and fox-specific DNA hybridisation probes identified a genomic sized 3.3-kb mRNA and a subgenomic 2.2-kb messenger RNA. Using a 5'-gag hybridisation probe, only the genomic 3.3-kb RNA molecule was detected, demonstrating that a donor splice site is present upstream of the gag sequences and used to generate the fos-specific 2.2-kb subgenomic mRNA.

摘要

已知FBR鼠病毒复合体与FBJ鼠病毒复合体都是新生小鼠的骨肿瘤诱导剂。这两种转化病毒在其基因组中都转导了源自c-原癌基因fos的序列。FBR-MuSV作为一个具有生物活性的10kbp EcoRI片段,从非生产性转化的大鼠胚胎成纤维细胞中被分子克隆到Charon噬菌体4A(λMOL503)中,随后亚克隆到质粒pBR322(pMOL503)中。其天然相关的辅助病毒FBR-MuLV,作为一个8.2kbp的内部PstI前病毒DNA片段,从慢性感染的NIH/3T3细胞中切下,被克隆到pBR322的唯一PstI位点。对FBR-MuSV和FBR-MuLV的限制性图谱进行比较分析,以及对两个分子克隆之间形成的异源双链DNA分子进行电子显微镜分析,表明FBR-MuLV是FBR-MuSV的亲本病毒。fos和fox特异性DNA杂交探针鉴定出一个基因组大小的3.3kb mRNA和一个亚基因组的2.2kb信使RNA。使用5'-gag杂交探针,只检测到基因组3.3kb的RNA分子,这表明在gag序列上游存在一个供体剪接位点,并用于产生fos特异性的2.2kb亚基因组mRNA。

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