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痘苗病毒基因组左端转录和翻译图谱扩展至21千碱基对。

Extension of the transcriptional and translational map of the left end of the vaccinia virus genome to 21 kilobase pairs.

作者信息

Cooper J A, Wittek R, Moss B

出版信息

J Virol. 1981 Sep;39(3):733-45. doi: 10.1128/JVI.39.3.733-745.1981.

Abstract

Physical, transcriptional, and translational maps of an EcoRI fragment located between 15,800 and 20,600 base pairs from the left end of the vaccinia virus genome were prepared. Major polypeptides with molecular weights of 14,000 (14K polypeptide), 32,000 and 38,000 were synthesized in a reticulocyte cell-free system programmed with immediate early RNA made in the presence of cycloheximide and selected by hybridization to lambda recombinant DNA containing the EcoRI fragment. With early RNA made in the presence of cytosine arabinoside, an inhibitor of DNA replication, the polypeptide pattern was similar except for quantitative differences in which less 38K polypeptide was detected as a translation product. With late RNA, isolated 6 h after infection without inhibitors, only traces of the early translation products were found and a new 40K polypeptide was detected. The size of the mRNA's for the 14K, 32K, and 38K polypeptides were determined to be approximately 760,880, and 1,150 nucleotides, respectively, by several independent procedures. Several large early RNAs not shown to code for any additional translation products were also detected. The size of the late message for the 40K polypeptide varied from 920 to 3,100 nucleotides. This heterogeneity appeared to be a general property of vaccinia virus late mRNA's. No evidence of RNA splicing was obtained by analysis of RNA-DNA hybrids after nuclease S1 treatment. Further analyses using separated recombinant DNA strands and restriction fragments indicated that all mRNA's were encoded by the leftward-reading DNA strand and at least two were overlapping. Since early and late mRNA's were encoded by the same DNA strand, the possibility of temporal regulation by transcriptional strand switching was eliminated. In conjunction with previous studies, a transcriptional map of the left 20,600 base pairs of the vaccinia virus genome was derived.

摘要

制备了痘苗病毒基因组左端15800至20600碱基对之间的EcoRI片段的物理图谱、转录图谱和翻译图谱。分子量分别为14000(14K多肽)、32000和38000的主要多肽是在网织红细胞无细胞系统中合成的,该系统用在放线菌酮存在下产生的立即早期RNA进行编程,并通过与含有EcoRI片段的λ重组DNA杂交进行筛选。用DNA复制抑制剂阿糖胞苷存在下产生的早期RNA时,多肽模式相似,只是在翻译产物中检测到的38K多肽数量较少,存在定量差异。用感染后6小时在无抑制剂情况下分离的晚期RNA时,仅发现少量早期翻译产物,并检测到一种新的40K多肽。通过几种独立的方法确定,14K、32K和38K多肽的mRNA大小分别约为760、880和1150个核苷酸。还检测到几种未显示编码任何其他翻译产物的大型早期RNA。40K多肽的晚期信使RNA大小在920至3100个核苷酸之间变化。这种异质性似乎是痘苗病毒晚期mRNA的普遍特性。核酸酶S1处理后分析RNA-DNA杂交体未获得RNA剪接的证据。使用分离的重组DNA链和限制性片段的进一步分析表明,所有mRNA均由向左阅读的DNA链编码,并且至少有两个是重叠的。由于早期和晚期mRNA由同一条DNA链编码,因此消除了转录链切换进行时间调控的可能性。结合先前的研究,得出了痘苗病毒基因组左侧20600碱基对的转录图谱。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c089/171307/b6d625a1a1e3/jvirol00009-0081-a.jpg

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