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Tetralin-Induced and ThnR-Regulated Aldehyde Dehydrogenase and β-Oxidation Genes in Sphingomonas macrogolitabida Strain TFA

机译:四氟鞘氨醇单胞菌TFA的Tetralin诱导和ThnR调节醛脱氢酶和β氧化基因。

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摘要

A new cluster of genes has been found downstream of the previously identified thnA2 gene. The gene products are similar to nonacylating aldehyde dehydrogenases (ThnG) and to proteins representing a complete β-oxidation pathway (ThnH to ThnP). ThnG has a nonacylating NAD-dependent pimelic semialdehyde dehydrogenase activity that renders pimelic acid a seven-carbon dicarboxylic acid. For further metabolism via β-oxidation, pimelic acid could be acylated by a constitutive acyl coenzyme A (acyl-CoA) ligase found in Sphingomonas macrogolitabida strain TFA or by ThnH, which would transfer CoA from a previously acylated molecule. The first round of β-oxidation is expected to render glutaryl-CoA and acetyl-CoA. Glutaryl-CoA dehydrogenase (ThnN) would catalyze the oxidation and decarboxylation of glutaryl-CoA and yield crotonyl-CoA, which enters the central metabolism via acetyl-CoA. Mutagenesis studies have shown that these genes are not essential for growth on tetralin or fatty acids, although a thnG disruption mutant showed threefold less pimelic semialdehyde dehydrogenase activity. Transcriptional analysis indicated that these genes are induced by tetralin, subjected to catabolite repression, and regulated by the same regulatory factors previously identified to regulate other thn structural genes. In the present study, transcription initiation upstream of thnH and thnM has been detected by primer extension analysis, and putative promoters were identified by sequence analysis. In addition, binding of the activator ThnR to its putative binding sites at the PH and PM promoter regions has been characterized. These results provide a complete characterization of the biodegradation pathway of tetralin to central metabolites and describe the transcriptional organization of the thn operons in S. macrogolitabida strain TFA.
机译:在先前鉴定的thnA2基因的下游发现了新的基因簇。基因产物类似于非酰化醛脱氢酶(ThnG)和代表完整的β-氧化途径的蛋白(ThnH到ThnP)。 ThnG具有非酰化NAD依赖性庚二酸半醛脱氢酶活性,使庚二酸成为七碳二羧酸。为了通过β-氧化作用进一步代谢,庚二酸可以通过鞘脂单胞菌(Sphingomonas macrogolitabida)菌株TFA中发现的组成型酰基辅酶A(酰基-CoA)连接酶或ThnH进行酰化,后者将从先前酰化的分子中转移CoA。预计第一轮β-氧化将产生戊二酰-CoA和乙酰基-CoA。戊二酰辅酶A脱氢酶(ThnN)将催化戊二酰辅酶A的氧化和脱羧并产生巴豆酰辅酶A,其通过乙酰辅酶A进入中心代谢。诱变研究表明,尽管thnG破坏突变体显示出的庚二酸半醛脱氢酶活性降低了三倍,但这些基因对于在四氢化萘或脂肪酸上生长并不是必需的。转录分析表明,这些基因是由四氢萘诱导的,经历了分解代谢物的阻遏作用,并由先前鉴定出的调​​控其他thn结构基因的相同调控因子调控。在本研究中,已通过引物延伸分析检测到thnH和thnM上游的转录起始,并通过序列分析鉴定了推定的启动子。另外,已经表征了活化剂ThnR与其在PH和PM启动子区域的假定结合位点的结合。这些结果提供了四氢化萘到中心代谢物的生物降解途径的完整表征,并描述了在大果链霉菌TFA菌株中thn操纵子的转录组织。

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