首页> 外文期刊>Korean Journal of Microbiology and Biotechnology >Comparative Analysis of Aniline Dioxygenase Genes from Aniline Degrading Bacteria, Burkholderia sp. HY1 and Delftia sp. HY99
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Comparative Analysis of Aniline Dioxygenase Genes from Aniline Degrading Bacteria, Burkholderia sp. HY1 and Delftia sp. HY99

机译:苯胺降解细菌伯克霍尔德氏菌苯胺双加氧酶基因的比较分析。 HY1和Delftia sp。 HY99

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In this study, aniline dioxygenase genes responsible for initial catabolism of aniline in Burkholderia sp. HY1 and Delftia sp. HY99 were cloned and the amino acid sequences were comparatively analyzed, which already have been reported as bacteria utilizing aniline as a sole source of carbon and nitrogen, B. sp. HY1 was found to have at least a plasmid, and the plasmid-cured strain, B. sp. HY1-PC obtained using mitomycin C was tested with wild type strain to investigate whether the former maintained the degradability for aniline. This proved that the aniline oxygenase gene from B. sp. HY1 was located in chromosomal DNA, not in plasmid DNA. Aniline dioxygenase small subunits from B. sp. HY1 and D. sp. HY99 were found, based on 146 amino acids, to share 79% similarity. Notably, ado2 genes from B. sp. HY1 andD. sp. HY99 which were found to be terminal dioxygenase of aniline dioxygenase small subunit showed 99% similarity in the deduced amino acid sequences with tdnA2 of Fmteuria sp. ANA-18 and danA2 ofD. sp. AN3, respectively. Besides, enzyme assay and amino acid sequence analysis of catechol dioxygenase supported the previous report that B. sp. HY1 might occupy ortho-cleavage pathway using catechol 1,2-diox-ygenase, while D. sp. HY99 might occupy catechol 2,3-dioxygenase for meto-cleavage pathway.
机译:在这项研究中,苯胺双加氧酶基因负责Burkholderia sp。中苯胺的初始分解代谢。 HY1和Delftia sp。克隆了HY99并比较了氨基酸序列,已报道它们是利用苯胺作为唯一碳和氮源的细菌。发现HY1至少具有一个质粒,以及该质粒固化的菌株B.sp。用丝裂霉素C获得的HY1-PC用野生型菌株进行测试,以研究前者是否保持了苯胺的降解性。这证明了来自B.sp.的苯胺氧化酶基因。 HY1位于染色体DNA中,而不位于质粒DNA中。来自B.sp.的苯胺双加氧酶小亚基。 HY1和D.sp.基于146个氨基酸,发现HY99具有79%的相似性。值得注意的是,来自芽孢杆菌的ado2基因。 HY1和D。 sp。被认为是苯胺双加氧酶小亚基的末端双加氧酶的HY99在推导的氨基酸序列中与Fmteuria sp。的tdnA2具有99%的相似性。 D的ANA-18和danA2。 sp。 AN3。此外,儿茶酚双加氧酶的酶法测定和氨基酸序列分析支持了以前的报道。 HY1可能使用邻苯二酚1,2-二氧合酶产生邻位裂解途径,而D. sp。 HY99可能占据儿茶酚2,3-二加氧酶的Meto裂解途径。

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