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A hydrogen-sensing system in transcriptional regulation of hydrogenase gene expression in Alcaligenes species.

机译:一个氢感测系统,用于调控产碱菌物种中氢化酶基因表达的转录。

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摘要

Heterologous complementation studies using Alcaligenes eutrophus H16 as a recipient identified a hydrogenase-specific regulatory DNA region on megaplasmid pHG21-a of the related species Alcaligenes hydrogenophilus. Nucleotide sequence analysis revealed four open reading frames on the subcloned DNA, designated hoxA, hoxB, hoxC, and hoxJ. The product of hoxA is homologous to a transcriptional activator of the family of two-component regulatory systems present in a number of H2-oxidizing bacteria. hoxB and hoxC predict polypeptides of 34.5 and 52.5 kDa, respectively, which resemble the small and the large subunits of [NiFe] hydrogenases and correlate with putative regulatory proteins of Bradyrhizobium japonicum (HupU and HupV) and Rhodobacter capsulatus (HupU). hoxJ encodes a protein with typical consensus motifs of histidine protein kinases. Introduction of the complete set of genes on a broad-host-range plasmid into A. eutrophus H16 caused severe repression of soluble and membrane-bound hydrogenase (SH and MBH, respectively) synthesis in the absence of H2. This repression was released by truncation of hoxJ. H2-dependent hydrogenase gene transcription is a typical feature of A. hydrogenophilus and differs from the energy and carbon source-responding, H2-independent mode of control characteristic of A. eutrophus H16. Disruption of the A. hydrogenophilus hoxJ gene by an in-frame deletion on megaplasmid pHG21-a led to conversion of the regulatory phenotype: SH and MBH of the mutant were expressed in the absence of H2 in response to the availability of the carbon and energy source. RNA dot blot analysis showed that HoxJ functions on the transcriptional level. These results suggest that the putative histidine protein kinase HoxJ is involved in sensing molecular hydrogen, possibly in conjunction with the hydrogenase-like polypeptides HoxB and HoxC.
机译:使用嗜碱拟南芥H16作为受体的异源互补研究鉴定了相关物种嗜碱嗜碱菌的大质粒pHG21-a上的氢化酶特异性调节DNA区域。核苷酸序列分析揭示了亚克隆DNA上的四个开放阅读框,命名为hoxA,hoxB,hoxC和hoxJ。 hoxA的产物与存在于许多H2氧化细菌中的两组分调节系统家族的转录激活因子同源。 hoxB和hoxC预测的多肽分别为34.5和52.5 kDa,类似于[NiFe]氢化酶的小亚基和大亚基,并与日本根瘤菌(HupU和HupV)和荚膜红细菌(HupU)的推定调节蛋白相关。 hoxJ编码一种具有组氨酸蛋白激酶典型共有基序的蛋白。在宽宿主范围的质粒上将完整的基因导入真人曲霉H16,导致在不存在H2的情况下严重抑制了可溶性和膜结合氢酶(分别为SH和MBH)的合成。此抑制是通过hoxJ的截断而释放的。 H2依赖的加氢酶基因转录是嗜氢假单胞菌的一个典型特征,它不同于真核曲霉H16的能量和碳源响应,H2独立的控制模式。通过大质粒pHG21-a的框内缺失破坏嗜水链球菌hoxJ基因,导致调节表型转换:突变体的SH和MBH在不存在H2的情况下表达,以响应碳和能量的利用资源。 RNA点印迹分析表明,HoxJ在转录水平上起作用。这些结果表明推定的组氨酸蛋白激酶HoxJ可能与氢化酶样多肽HoxB和HoxC一起参与分子氢感测。

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