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苜蓿中华根瘤菌1021在转变至酸性pH值后转录组反应的时间进程。

The time course of the transcriptomic response of Sinorhizobium meliloti 1021 following a shift to acidic pH.

作者信息

Hellweg Christoph, Pühler Alfred, Weidner Stefan

机构信息

Lehrstuhl für Genetik, Fakultät für Biologie, Universität Bielefeld, Bielefeld, Germany.

出版信息

BMC Microbiol. 2009 Feb 15;9:37. doi: 10.1186/1471-2180-9-37.

Abstract

BACKGROUND

The symbiotic soil bacterium Sinorhizobium meliloti often has to face low pH in its natural habitats. To identify genes responding to pH stress a global transcriptional analysis of S. meliloti strain 1021 following a pH shift from pH 7.0 to pH 5.75 was carried out. In detail, oligo-based whole genome microarrays were used in a time course experiment. The monitoring period covered a time span of about one hour after the pH shift. The obtained microarray data was filtered and grouped by K-means clustering in order to obtain groups of genes behaving similarly concerning their expression levels throughout the time course.

RESULTS

The results display a versatile response of S. meliloti 1021 represented by distinct expression profiles of subsets of genes with functional relation. The eight generated clusters could be subdivided into a group of four clusters containing genes that were up-regulated and another group of four clusters containing genes that were down-regulated in response to the acidic pH shift. The respective mean expression progression of the four up-regulated clusters could be described as (i) permanently and strong, (ii) permanently and intermediate, (iii) permanently and progressive, and (iv) transiently up-regulated. The expression profile of the four down-regulated clusters could be characterized as (i) permanently, (ii) permanently and progressive, (iii) transiently, and (iv) ultra short down-regulated. Genes coding for proteins with functional relation were mostly cumulated in the same cluster, pointing to a characteristic expression profile for distinct cellular functions. Among the strongest up-regulated genes lpiA, degP1, cah, exoV and exoH were found. The most striking functional groups responding to the shift to acidic pH were genes of the exopolysaccharide I biosynthesis as well as flagellar and chemotaxis genes. While the genes of the exopolysaccharide I biosynthesis (exoY, exoQ, exoW, exoV, exoT, exoH, exoK exoL, exoO, exoN, exoP) were up-regulated, the expression level of the flagellar and chemotaxis genes (visR, motA, flgF, flgB, flgC, fliE, flgG, flgE, flgL, flbT, mcpU) simultaneously decreased in response to acidic pH. Other responding functional groups of genes mainly belonged to nitrogen uptake and metabolism (amtB, nrtB, nirB, nirD), methionine metabolism (metA, metF, metH, metK, bmt and ahcY) as well as ion transport systems (sitABCD, phoCD). It is noteworthy, that several genes coding for hypothetical proteins of unknown function could be identified as up-regulated in response to the pH shift.

CONCLUSION

It was shown that the short term response to acidic pH stress does not result in a simple induction or repression of genes, but in a sequence of responses varying in their intensity over time. Obviously, the response to acidic pH is not based on a few specific genes, but involves whole sets of genes associated with various cellular functions.

摘要

背景

共生土壤细菌苜蓿中华根瘤菌在其自然栖息地中常常面临低pH环境。为了鉴定对pH胁迫有响应的基因,对苜蓿中华根瘤菌1021菌株在pH从7.0转变为5.75后的全局转录情况进行了分析。具体而言,在一个时间进程实验中使用了基于寡核苷酸的全基因组微阵列。监测期涵盖了pH转变后约一小时的时间跨度。所获得的微阵列数据经过筛选并通过K均值聚类进行分组,以便获得在整个时间进程中表达水平表现相似的基因群组。

结果

结果显示苜蓿中华根瘤菌1021呈现出多方面的响应,由具有功能关联的基因子集的不同表达谱所代表。所生成的八个聚类可细分为一组包含上调基因的四个聚类和另一组包含下调基因的四个聚类,这些基因是对酸性pH转变做出响应的。四个上调聚类各自的平均表达进程可描述为:(i)持续且强烈上调,(ii)持续且中等上调,(iii)持续且渐进上调,以及(iv)短暂上调。四个下调聚类的表达谱可表征为:(i)持续下调,(ii)持续且渐进下调,(iii)短暂下调,以及(iv)极短暂下调。编码具有功能关联蛋白质的基因大多聚集在同一聚类中,表明不同细胞功能具有特征性的表达谱。在上调最强烈的基因中发现了lpiA、degP1、cah、exoV和exoH。对向酸性pH转变做出响应的最显著功能组是胞外多糖I生物合成基因以及鞭毛和趋化性基因。虽然胞外多糖I生物合成基因(exoY、exoQ、exoW、exoV、exoT、exoH、exoK、exoL、exoO、exoN、exoP)被上调,但鞭毛和趋化性基因(visR、motA、flgF、flgB、flgC、fliE、flgG、flgE、flgL、flbT、mcpU)的表达水平同时因酸性pH而降低。其他做出响应的基因功能组主要属于氮吸收和代谢(amtB、nrtB、nirB、nirD)、甲硫氨酸代谢(metA, metF, metH, metK, bmt和ahcY)以及离子转运系统(sitABCD、phoCD)。值得注意的是,几个编码功能未知的假设蛋白的基因被鉴定为对pH转变有上调响应。

结论

结果表明,对酸性pH胁迫的短期响应并非导致基因的简单诱导或抑制,而是一系列随时间强度变化的响应。显然,对酸性pH的响应并非基于少数特定基因,而是涉及与各种细胞功能相关的整套基因。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7d25/2651895/3c5c97b91296/1471-2180-9-37-1.jpg

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