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首页> 外文期刊>Environmental microbiology >Genes encoding the candidate enzyme for anaerobic activation of n-alkanes in the denitrifying bacterium, strain HxN1
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Genes encoding the candidate enzyme for anaerobic activation of n-alkanes in the denitrifying bacterium, strain HxN1

机译:编码脱氮细菌HxN1菌株中正构烷烃厌氧活化候选酶的基因

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Strain HxN1, a member of the Betaproteobacteria, can grow anaerobically by denitrification with n-alkanes. n-Alkanes are apparently activated by subterminal carbon addition to fumarate yielding (1-methylalkyl)succinates, the postulated enzyme being (1-methylalkyl)succinate synthase (Mas). Genes encoding this enzyme (mas) were searched for via proteins that were specifically formed in n-hexane-grown cells (in comparison with caproate-grown cells), as revealed by two-dimensional gel electrophoresis. Partial amino acid sequencing and subsequent probe development for hybridization of restricted DNA led to the identification of a gene cluster. Deduced proteins are similar to the subunits of benzylsuccinate synthase (Bss), the toluene-activating enzyme in other anaerobic bacteria and its activase. The tentative (1-methylalkyl)succinate synthase is presumably a heterotrimer (MasDEC) which, like benzylsuccinate synthase, contains a motif (in MasD, the large subunit) characteristic of glycyl radical-bearing sites. Based on amino acid sequence comparison, the tentative (1-methylalkyl)succinate synthase branches outside of the phylogenetic cluster of benzylsuccinate synthases from different organisms and represents a separate line of descent within glycyl radical enzymes. n-Hexane-induced co-transcription of the mas genes and additional genes of an apparent operon was demonstrated by Northern hybridization experiments.
机译:HxN1菌株是Betaproteobacteria的成员,可以通过正构烷烃的反硝化而厌氧生长。正构烷烃显然是通过向富马酸酯的亚末端碳加成而活化的,从而生成(1-甲基烷基)琥珀酸酯,假定的酶是(1-甲基烷基)琥珀酸酯合酶(Mas)。如二维凝胶电泳所示,通过在正己烷生长的细胞(与己酸生长的细胞相比)中特异性形成的蛋白质,搜索编码该酶(mas)的基因。部分氨基酸测序和随后用于限制性DNA杂交的探针开发导致了基因簇的鉴定。推导的蛋白质类似于琥珀酸苄基合酶(Bss)的亚基,其他厌氧细菌中的甲苯活化酶及其活化酶。暂定的(1-甲基烷基)琥珀酸合酶可能是异源三聚体(MasDEC),与苄基琥珀酸合酶一样,它含有带有糖基的位点特征的基序(在MasD中为大的亚基)。基于氨基酸序列比较,暂定的(1-甲基烷基)琥珀酸合酶分支在来自不同生物体的琥珀酸苄基合酶的系统发生簇之外,并且代表了糖基自由基酶中的一个单独的下降系。北部杂交实验证明了正己烷诱导的mas基因和其他操纵子基因的共转录。

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