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PhaD 调控子控制着参与聚羟基烷酸代谢和周转的 pha 基因在恶臭假单胞菌 KT2442 中的同时表达。

The PhaD regulator controls the simultaneous expression of the pha genes involved in polyhydroxyalkanoate metabolism and turnover in Pseudomonas putida KT2442.

机构信息

Environmental Biology Department, Centro de Investigaciones Biológicas, CSIC, Ramiro de Maeztu, 9, 28040 Madrid, Spain.

出版信息

Environ Microbiol. 2010 Jun;12(6):1591-603. doi: 10.1111/j.1462-2920.2010.02199.x. Epub 2010 Apr 14.

DOI:10.1111/j.1462-2920.2010.02199.x
PMID:20406286
Abstract

The promoters of the pha gene cluster encoding the enzymes involved in the metabolism of polyhydroxyalkanoates (PHAs) in the model strain Pseudomonas putida KT2442 have been identified and compared. The pha locus is composed by five functional promoters upstream the phaC1, phaZ, phaC2, phaF and phaI genes (P(C1), P(Z), P(C2), P(F) and P(I) respectively). P(C1) and P(I) are the most active promoters of the pha cluster allowing the transcription of phaC1ZC2D and phaIF operons. All promoters with the sole exception of P(F) are carbon source-dependent. Their transcription profiles explain the simultaneous production of PHA depolymerase and synthases to maintain the metabolic balance and PHA turnover. Mutagenesis analyses demonstrated that PhaD, a TetR-like transcriptional regulator, behaves as a carbon source-dependent activator of the pha cluster. The phaD gene is mainly transcribed as part of the phaC1ZC2D transcription unit and controls its own transcription and that of phaIF operon. The ability of PhaD to bind the P(C1) and P(I) promoters was analysed by gel retardation and DNase I footprinting assays, demonstrating that PhaD interacts with a region of 25 bp at P(C1) promoter (named OPRc1) and a 29 bp region at P(I) promoter (named OPRi). These operators contain a single binding site formed by two inverted half sites of 6 bp separated by 8 bp which overlap the corresponding promoter boxes. The 3D model structure of PhaD activator predicts that the true effector might be a CoA-intermediate of fatty acid beta-oxidation.

摘要

已鉴定并比较了编码聚羟基烷酸(PHA)代谢酶的pha 基因簇在模式菌株恶臭假单胞菌 KT2442 中各启动子。pha 基因座由 phaC1、phaZ、phaC2、phaF 和 phaI 基因上游的五个功能启动子组成(分别为 P(C1)、P(Z)、P(C2)、P(F)和 P(I))。P(C1)和 P(I)是 pha 簇中最活跃的启动子,允许 phaC1ZC2D 和 phaIF 操纵子的转录。除了 P(F)之外,所有启动子都是碳源依赖性的。它们的转录谱解释了同时产生 PHA 解聚酶和合成酶以维持代谢平衡和 PHA 周转。突变分析表明,TetR 样转录调节因子 PhaD 是碳源依赖性的 pha 簇激活剂。phaD 基因主要作为 phaC1ZC2D 转录单元的一部分转录,并控制其自身的转录和 phaIF 操纵子的转录。凝胶阻滞和 DNase I 足迹分析表明,PhaD 能够结合 P(C1)和 P(I)启动子,分析了 PhaD 与 P(C1)启动子上 25 bp 区域(命名为 OPRc1)和 P(I)启动子上 29 bp 区域(命名为 OPRi)的相互作用。这些操作子包含由 6 bp 组成的单个结合位点,间隔 8 bp,重叠相应的启动子盒,该结合位点由脂肪酸β-氧化的 CoA 中间产物形成。PhaD 激活剂的 3D 模型结构预测,真正的效应物可能是脂肪酸β-氧化的 CoA 中间产物。

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