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绘制大肠杆菌链霉素操纵子 mRNA 上核糖体蛋白 S7 调节结合位点。

Mapping the ribosomal protein S7 regulatory binding site on mRNA of the E. coli streptomycin operon.

机构信息

Belozersky Institute of Physico-Chemical Biology, Lomonosov Moscow State University, Moscow, Russia.

出版信息

Biochemistry (Mosc). 2010 Jul;75(7):841-50. doi: 10.1134/s0006297910070059.

Abstract

In this work it is shown by deletion analysis that an intercistronic region (ICR) approximately 80 nucleotides in length is necessary for interaction with recombinant E. coli S7 protein (r6hEcoS7). A model is proposed for the interaction of S7 with two ICR sites-region of hairpin bifurcations and Shine-Dalgarno sequence of cistron S7. A de novo RNA binding site for heterologous S7 protein of Thermus thermophilus (r6hTthS7) was constructed by selection of a combinatorial RNA library based on E. coli ICR: it has only a single supposed protein recognition site in the region of bifurcation. The SERW technique was used for selection of two intercistronic RNA libraries in which five nucleotides of a double-stranded region, adjacent to the bifurcation, had the randomized sequence. One library contained an authentic AG (-82/-20) pair, while in the other this pair was replaced by AU. A serwamer capable of specific binding to r6hTthS7 was selected; it appeared to be the RNA68 mutant with eight nucleotide mutations. The serwamer binds to r6hTthS7 with the same affinity as homologous authentic ICR of str mRNA binds to r6hEcoS7; apparent dissociation constants are 89 +/- 43 and 50 +/- 24 nM, respectively.

摘要

在这项工作中,通过缺失分析表明,长约 80 个核苷酸的顺式间区(ICR)对于与重组大肠杆菌 S7 蛋白(r6hEcoS7)的相互作用是必要的。提出了一个 S7 与两个 ICR 位点——发夹分叉区域和 S7 顺式基因的 Shine-Dalgarno 序列相互作用的模型。通过基于大肠杆菌 ICR 的组合 RNA 文库的选择,构建了新型热球菌 S7 蛋白(r6hTthS7)的从头 RNA 结合位点:在分叉区域只有一个假定的蛋白质识别位点。SERW 技术用于选择两个顺式间 RNA 文库,其中双链区域的五个核苷酸,靠近分叉,具有随机序列。一个文库包含一个真实的 AG(-82/-20)对,而在另一个文库中,这个对被 AU 取代。选择了一个能够特异性结合 r6hTthS7 的 serwamer;它似乎是具有八个核苷酸突变的 RNA68 突变体。serwamer 与 r6hTthS7 的结合亲和力与同源性真实 ICR 与 r6hEcoS7 的结合亲和力相同;表观解离常数分别为 89 +/- 43 和 50 +/- 24 nM。

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