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使用平铺微阵列分析大肠杆菌 RNase E 和 RNase III 的体内活性。

Analysis of Escherichia coli RNase E and RNase III activity in vivo using tiling microarrays.

机构信息

Department of Genetics, University of Georgia, Athens, GA 30605, USA.

出版信息

Nucleic Acids Res. 2011 Apr;39(8):3188-203. doi: 10.1093/nar/gkq1242. Epub 2010 Dec 11.

Abstract

Tiling microarrays have proven to be a valuable tool for gaining insights into the transcriptomes of microbial organisms grown under various nutritional or stress conditions. Here, we describe the use of such an array, constructed at the level of 20 nt resolution for the Escherichia coli MG1655 genome, to observe genome-wide changes in the steady-state RNA levels in mutants defective in either RNase E or RNase III. The array data were validated by comparison to previously published results for a variety of specific transcripts as well as independent northern analysis of additional mRNAs and sRNAs. In the absence of RNase E, 60% of the annotated coding sequences showed either increases or decreases in their steady-state levels. In contrast, only 12% of the coding sequences were affected in the absence of RNase III. Unexpectedly, many coding sequences showed decreased abundance in the RNase E mutant, while more than half of the annotated sRNAs showed changes in abundance. Furthermore, the steady-state levels of many transcripts showed overlapping effects of both ribonucleases. Data are also presented demonstrating how the arrays were used to identify potential new genes, RNase III cleavage sites and the direct or indirect control of specific biological pathways.

摘要

平铺式微阵列已被证明是一种非常有价值的工具,可用于深入了解在各种营养或应激条件下生长的微生物生物体的转录组。在这里,我们描述了此类微阵列的使用,该微阵列在大肠杆菌 MG1655 基因组的 20nt 分辨率水平上构建,用于观察 RNase E 或 RNase III 缺陷突变体中稳定态 RNA 水平的全基因组变化。通过与各种特定转录物的先前发表结果以及对其他 mRNA 和 sRNA 的独立 northern 分析进行比较,验证了阵列数据。在没有 RNase E 的情况下,60%的注释编码序列的稳定态水平要么增加,要么减少。相比之下,在没有 RNase III 的情况下,只有 12%的编码序列受到影响。出乎意料的是,许多编码序列在 RNase E 突变体中丰度降低,而超过一半的注释 sRNA 丰度发生变化。此外,许多转录物的稳定态水平表现出两种核酶的重叠效应。还提供了数据,证明了如何使用阵列来识别潜在的新基因、RNase III 切割位点以及特定生物途径的直接或间接控制。

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