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核糖核酸酶III对噬菌体T7溶菌酶信使核糖核酸翻译效率的影响。

Effect of RNase III on efficiency of translation of bacteriophage T7 lysozyme mRNA.

作者信息

Hagen F S, Young E T

出版信息

J Virol. 1978 Jun;26(3):793-804. doi: 10.1128/JVI.26.3.793-804.1978.

Abstract

RNase III had no positive effect on the translation of bacteriophage T7 lysozyme mRNA in vivo or in vitro. The time of appearance and quanity of lysozyme in T7-infected E. coli BL107, an RNase III- strain, and T7-infected E. coli BL15, a nearly isogenic RNase III+ strain, were indistinguishable. Nearly identical patterns of lysozyme mRNA activity were obtained when RNA extracted at different times after infection of RNase III+ and RNase III- hosts was translated in cell-free extracts of E. coli containing or lacking RNase III. Exposure of RNA extracted from T7-infected E. coli BL107 (RNase III-) to purified RNase III did not increase the lysozyme mRNA activity of this RNA. The only result that implied that RNase III has a differential effect on the translatability of the lysozyme mRNA was the translation of fractionaed RNA from T7-infected E. coli BL107. Translation of the smallest and largest lysozyme messages, 0.33 x 10(6) and 4 x 10(6) to 5 x 10(6) daltons, was the most inefficient in RNase III- cell-free extracts as compared to RNase III+ cell-free translation. The translation of the most abundant, medium-sized lysozyme mRNA between 0.9 x 10(6) and 1.5 x 10(6) daltons was the least affected by the absence of RNase III. The existence of a lag between the appearance of lysozyme mRNA and the appearance of lysozyme in T7 infection was confirmed. In these studies a very rapid method of RNA extraction was used, eliminating the possibility of continued RNA transcription during cell collection and RNA extraction. With this method of analysis, the length of the lag period was established at about 3 min. The possibility that RNase III is the controlling element of the lag period was eliminated by these investigations.

摘要

核糖核酸酶III(RNase III)对噬菌体T7溶菌酶信使核糖核酸(mRNA)的体内或体外翻译均无积极作用。在感染T7的大肠杆菌BL107(一种缺乏RNase III的菌株)和感染T7的大肠杆菌BL15(一种近乎同基因的RNase III+菌株)中,溶菌酶出现的时间和数量并无差异。当在含有或缺乏RNase III的大肠杆菌无细胞提取物中翻译感染RNase III+和RNase III-宿主后不同时间提取的RNA时,获得了几乎相同的溶菌酶mRNA活性模式。将从感染T7的大肠杆菌BL107(RNase III-)中提取的RNA暴露于纯化的RNase III中,并未提高该RNA的溶菌酶mRNA活性。唯一表明RNase III对溶菌酶mRNA的可翻译性有差异影响的结果是对感染T7的大肠杆菌BL107的分级RNA的翻译。与RNase III+无细胞翻译相比,在RNase III-无细胞提取物中,最小和最大的溶菌酶信使核糖核酸(分别为0.33×10⁶和4×10⁶至5×10⁶道尔顿)的翻译效率最低。在0.9×10⁶至1.5×10⁶道尔顿之间最丰富的中等大小溶菌酶mRNA的翻译受RNase III缺失的影响最小。证实了在T7感染中溶菌酶mRNA出现与溶菌酶出现之间存在延迟。在这些研究中,使用了一种非常快速的RNA提取方法,排除了细胞收集和RNA提取过程中持续RNA转录的可能性。通过这种分析方法,确定延迟期约为3分钟。这些研究排除了RNase III是延迟期控制元件的可能性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/32ef/525904/05c3fe172ccd/jvirol00198-0261-a.jpg

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