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利用染色质免疫沉淀法确定球形红杆菌2.4.1中PpsR的结合活性

The use of chromatin immunoprecipitation to define PpsR binding activity in Rhodobacter sphaeroides 2.4.1.

作者信息

Bruscella Patrice, Eraso Jesus M, Roh Jung Hyeob, Kaplan Samuel

机构信息

Department of Microbiology and Molecular Genetics, University of Texas Health Science Center, Houston, TX 77030, USA.

出版信息

J Bacteriol. 2008 Oct;190(20):6817-28. doi: 10.1128/JB.00719-08. Epub 2008 Aug 8.

Abstract

The expression of genes involved in photosystem development in Rhodobacter sphaeroides is dependent upon three major regulatory networks: FnrL, the PrrBA (RegBA) two-component system, and the transcriptional repressor/antirepressor PpsR/AppA. Of the three regulators, PpsR appears to have the narrowest range of physiological effects, which are limited to effects on the structural and pigment biosynthetic activities involved in photosynthetic membrane function. Although a PrrA(-) mutant is unable to grow under photosynthetic conditions, when a ppsR mutation was present, photosynthetic growth occurred. An examination of the double mutant under anaerobic-dark-dimethyl sulfoxide conditions using microarray analysis revealed the existence of an "extended" PpsR regulon and new physiological roles. To characterize the PpsR regulon and to better ascertain the significance of degeneracy within the PpsR binding sequence in vivo, we adapted the chromatin immunoprecipitation technique to R. sphaeroides. We demonstrated that in vivo there was direct and significant binding by PpsR to newly identified genes involved in microaerobic respiration and periplasmic stress resistance, as well as to photosynthesis genes. The new members of the PpsR regulon are located outside the photosynthesis gene cluster and have degenerate PpsR binding sequences. The possible interaction under physiologic conditions with degenerate binding sequences in the presence of other biologically relevant molecules is discussed with respect to its importance in physiological processes and to the existence of complex phenotypes associated with regulatory mutants. This study further defines the DNA structure necessary for PpsR binding in situ.

摘要

球形红细菌中参与光系统发育的基因表达依赖于三个主要调控网络

FnrL、PrrBA(RegBA)双组分系统以及转录阻遏物/抗阻遏物PpsR/AppA。在这三种调控因子中,PpsR的生理效应范围似乎最窄,仅限于对光合膜功能中涉及的结构和色素生物合成活性的影响。虽然PrrA(-)突变体在光合条件下无法生长,但当存在ppsR突变时,光合生长就会发生。在厌氧 - 黑暗 - 二甲基亚砜条件下使用微阵列分析对双突变体进行检测,揭示了一个“扩展的”PpsR调控子以及新的生理作用。为了表征PpsR调控子并更好地确定体内PpsR结合序列内简并性的意义,我们将染色质免疫沉淀技术应用于球形红细菌。我们证明,在体内PpsR直接且显著地结合到新鉴定的参与微需氧呼吸和周质应激抗性的基因以及光合作用基因上。PpsR调控子的新成员位于光合作用基因簇之外,并且具有简并的PpsR结合序列。本文讨论了在生理条件下与简并结合序列在其他生物相关分子存在时可能的相互作用,涉及其在生理过程中的重要性以及与调控突变体相关的复杂表型的存在。这项研究进一步定义了PpsR原位结合所需的DNA结构。

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