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Biochemical Characterization of 3-Methyl-4-nitrophenol Degradation in Burkholderia sp Strain SJ98

机译:伯克霍尔德氏菌SJ98菌株3-甲基-4-硝基苯酚降解的生化特性

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摘要

Several strains have been reported to grow on 3-methyl-4-nitrophenol (3M4NP), the primary breakdown product of the excessively used insecticide fenitrothion. However, the microbial degradation of 3M4NP at molecular and biochemical levels remains unknown. Here, methyl-1,4-benzoquinone (MBQ) and methylhydroquinone (MHQ), rather than catechol proposed previously, were identified as the intermediates before ring cleavage during 3M4NP degradation by Burkholderia sp. strain SJ98. Realtime quantitative PCR analysis indicated that the pnpABA1CDEF cluster involved in para-nitrophenol (PNP) and 2-chloro-4-nitrophenol (2C4NP) catabolism was also likely responsible for 3M4NP degradation in this strain. Purified PNP 4-monooxygenase (PnpA) is able to catalyze the monooxygenation of 3M4NP to MBQ and exhibited an apparent K-m value of 20.3 +/- 2.54 mu M for 3M4NP, and pnpA is absolutely necessary for the catabolism of 3M4NP by gene knock-out and complementation. PnpB, a 1,4-benzoquinone reductase catalyzes the reduction of MBQ to MHQ, and also found to enhance PnpA activity in vitro in the conversion of 3M4NP to MBQ. By sequential catalysis assays, PnpCD, PnpE, and PnpF were likely involved in the lower pathway of 3M4NP catabolism. Although NpcCD, NpcE, and NpcF are able to catalyze the sequential conversion of MHQ in vitro, these enzymes are unlikely involved in 3M4NP catabolism because their coding genes were not upregulated by 3M4NP induction in vivo. These results revealed that the enzymes involved in PNP and 2C4NP catabolism were also responsible for 3M4NP degradation in strain SJ98. This fills a gap in our understanding of the microbial degradation of 3M4NP at molecular and biochemical levels and also provides another example to illustrate the adaptive flexibility in microbial catabolism for structurally similar compounds.
机译:据报道,几种菌株在3-甲基-4-硝基苯酚(3M4NP)上生长,3-甲基-4-硝基苯酚是过量使用的杀虫剂杀虫硫磷的主要分解产物。然而,在分子和生化水平上3M4NP的微生物降解仍然未知。在这里,而不是先前提出的儿茶酚,甲基-1,4-苯醌(MBQ)和甲基氢醌(MHQ)被确定为伯克霍尔德氏菌降解3M4NP降解环之前的中间体。菌株SJ98。实时定量PCR分析表明,参与对硝基苯酚(PNP)和2-氯-4-硝基苯酚(2C4NP)分解代谢的pnpABA1CDEF簇也可能是该菌株中3M4NP降解的原因。纯化的PNP 4-单加氧酶(PnpA)能够催化3M4NP到MBQ的单加氧反应,并显示3M4NP的表观Km值为20.3 +/- 2.54μM,而pnpA对于通过基因敲除进行3M4NP的分解代谢是绝对必要的和补充。 PnpB是一种1,4-苯醌还原酶,可催化将MBQ还原为MHQ,并且在3M4NP转化为MBQ的体外,还可增强PnpA的活性。通过顺序催化分析,PnpCD,PnpE和PnpF可能参与了3M4NP分解代谢的较低途径。尽管NpcCD,NpcE和NpcF能够在体外催化MHQ的顺序转化,但是这些酶不太可能参与3M4NP分解代谢,因为它们的编码基因在体内不会被3M4NP诱导上调。这些结果表明参与PNP和2C4NP分解代谢的酶也负责菌株SJ98中3M4NP的降解。这填补了我们对3M4NP在分子和生化水平上微生物降解的理解的空白,并且还提供了另一个例子来说明结构相似化合物在微生物分解代谢中的适应性灵活性。

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