首页> 外文OA文献 >Multiple-Subunit Genes of the Aromatic-Ring-Hydroxylating Dioxygenase Play an Active Role in Biphenyl and Polychlorinated Biphenyl Degradation in Rhodococcus sp. Strain RHA1
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Multiple-Subunit Genes of the Aromatic-Ring-Hydroxylating Dioxygenase Play an Active Role in Biphenyl and Polychlorinated Biphenyl Degradation in Rhodococcus sp. Strain RHA1

机译:芳香环加氢双加氧酶的多个亚基基因在红球菌中联苯和多氯联苯降解中发挥积极作用。菌株RHA1

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摘要

A gram-positive strong polychlorinated biphenyl (PCB) degrader, Rhodococcus sp. strain RHA1, can degrade PCBs by cometabolism with biphenyl or ethylbenzene. In RHA1, three sets of aromatic-ring-hydroxylating dioxygenase genes are induced by biphenyl. The large and small subunits of their terminal dioxygenase components are encoded by bphA1 and bphA2, etbA1 and etbA2, and ebdA1 and ebdA2, respectively, and the deduced amino acid sequences of etbA1 and etbA2 are identical to those of ebdA1 and ebdA2, respectively. In this study, we examined the involvement of the respective subunit genes in biphenyl/PCB degradation by RHA1. Reverse transcription-PCR and two-dimensional polyacrylamide gel electrophoresis analyses indicated the induction of RNA and protein products of etbA1 and ebdA1 by biphenyl. Single- and double-disruption mutants of etbA1, ebdA1, and bphA1 were constructed by insertional inactivation. The 4-chlorobiphenyl (4-CB) degradation activities of all the mutants were lower than that of RHA1. The results indicated that all of these genes are involved in biphenyl/PCB degradation. Furthermore, we constructed disruption mutants of ebdA3 and bphA3, encoding ferredoxin, and etbA4, encoding ferredoxin reductase components. The 4-CB degradation activities of these mutants were also lower than that of RHA1, suggesting that all of these genes play a role in biphenyl/PCB degradation. The substrate preferences of etbA1A2/ebdA1A2- and bphA1A2-encoded dioxygenases for PCB congeners were examined using the corresponding mutants. The results indicated that these dioxygenase isozymes have different substrate preferences and that the etbA1A2/ebdA1A2-encoded isozyme is more active on highly chlorinated congeners than the bphA1A2-encoded one.
机译:革兰氏阳性强多氯联苯(PCB)降解菌Rhodococcus sp。 RHA1菌株可通过与联苯或乙苯的代谢作用降解PCBs。在RHA1中,联苯诱导了三组芳香环-羟化双加氧酶基因。它们的末端双加氧酶组分的大亚基和小亚基分别由bphA1和bphA2,etbA1和etbA2以及ebdA1和ebdA2编码,并且etbA1和etbA2的推导氨基酸序列分别与ebdA1和ebdA2相同。在这项研究中,我们检查了RHA1参与联苯/ PCB降解的各个亚基基因的参与。逆转录PCR和二维聚丙烯酰胺凝胶电泳分析表明联苯诱导了etbA1和ebdA1的RNA和蛋白质产物。通过插入失活构建etbA1,ebdA1和bphA1的单干扰和双干扰突变体。所有突变体的4-氯联苯(4-CB)降解活性均低于RHA1。结果表明,所有这些基因都与联苯/ PCB降解有关。此外,我们构建了编码铁氧还蛋白的ebdA3和bphA3的破坏突变体,以及编码铁氧还蛋白还原酶成分的etbA4。这些突变体的4-CB降解活性也低于RHA1,表明所有这些基因均在联苯/ PCB降解中起作用。使用相应的突变体检查了etbA1A2 / ebdA1A2-和bphA1A2编码的双加氧酶对PCB同系物的底物偏好。结果表明,这些双加氧酶同工酶具有不同的底物偏好,并且与bphA1A2编码的同工酶相比,etbA1A2 / ebdA1A2编码的同工酶对高度氯化的同系物更具活性。

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