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首页> 外文期刊>Applied Microbiology >Differential Effects of Homologous Transcriptional Regulators NicR2A, NicR2B1, and NicR2B2 and Endogenous Ectopic Strong Promoters on Nicotine Metabolism in Pseudomonas sp. Strain JY-Q
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Differential Effects of Homologous Transcriptional Regulators NicR2A, NicR2B1, and NicR2B2 and Endogenous Ectopic Strong Promoters on Nicotine Metabolism in Pseudomonas sp. Strain JY-Q

机译:同源转录调节剂NICR2A,NICR2B1和NICR2B2和内源异位强促进剂对假单胞菌SP尼古丁代谢的差异效应。 菌株JY-Q

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Nicotine is a toxic environmental pollutant that widely exists in tobacco wastes. As a natural nicotine-degrading strain, Pseudomonas sp. strain JY-Q still has difficulties degrading high concentrations of nicotine. In this study, we investigated the effect of two homologous transcriptional regulators and endogenous ectopic strong promoters on the efficiency of nicotine degradation. Comparative genomics analysis showed that two homologous transcriptional regulators, namely, NicR2A and NicR2Bs (NicR2B1 plus NicR2B2), can repress nicotine degradation gene expression. When both nicR2A and nicR2Bs were deleted, the resulting mutant JY-Q Δ nicR2A Δ nicR2B1 Δ nicR2B2 (QΔABs) exhibits a 17% higher nicotine degradation efficiency than wild-type JY-Q. Transcriptome sequencing (RNA-seq) analysis showed that the transcription levels (fragments per kilobase per million [FPKM] value) of six genes were higher than those of the other genes in JY-Q. Based on the genetic organization of these genes, three putative promoters, P_(RS28250) , P_(RS09985) , and P_(RS24685) , were identified. Their promoter activities were evaluated by comparing their expression levels using reverse transcriptase quantitative PCR (RT-qPCR). We found that the transcription levels of RS28250 , RS09985 , and RS24685 were respectively 16.8, 2.6, and 1.6 times higher than that of hspB2 , encoding 6-hydroxy-3-succinylpyridine hydroxylase, which is involved in nicotine degradation. Thus, two strong endogenous promoters, namely, P_(RS28250) and P_(RS09985) , were selected to replace the original promoters of nic2 gene clusters. The effect of the endogenous ectopic promoter was also related to the position of target gene clusters. When the promoter P_(RS28250) replaced the promoter of hspB2 , the resultant mutant QΔABs-Δ P_(hspB2) :: P_(RS28250) exhibited nicotine-degrading efficiency 69% higher than that of JY-Q. This research suggests a feasible strategy to enhance strains' capacity for nicotine degradation by removal of repressing regulatory proteins and replacing the target promoter with strong endogenous ectopic promoters.IMPORTANCE This study evaluated the differential effects of homologous NicR2A and NicR2Bs and endogenous ectopic strong promoters on nicotine metabolism in Pseudomonas sp. strain JY-Q. Based on our differential analysis, a feasible strategy is presented to modify wild-type (WT) strain JY-Q by removing repressing regulatory proteins NicR2A and NicR2Bs and replacing the target promoter with strong endogenous ectopic promoters. The resulting mutants exhibited high tolerance and degradation of nicotine. These findings should be beneficial for improving the pollutant-degrading capacity of natural strains through genomic modification.
机译:尼古丁是一种毒性环境污染物,广泛存在于烟草废物中。作为天然尼古丁降解菌株,假单胞菌SP。菌株JY-Q仍然有困难降低高浓度的尼古丁。在这项研究中,我们研究了两种同源转录调节剂和内源异位强促进剂对尼古丁降解效率的影响。对比基因组学分析表明,两个同源转录调节剂,即NiCr2a和Nicr2bs(Nicr2b1加上NiCr2b2),可以抑制尼古丁降解基因表达。当缺失NICR2A和NICR2BS时,所得突变的JY-QδNICR2AδNICR2B1δNICR2B2(QΔAbs)比野生型JY-Q表现出17%的尼古丁劣化效率。转录组测序(RNA-SEQ)分析表明,六种基因的六种基因的转录水平(每百万百万[FPKM]值)高于JY-Q中的其他基因。基于这些基因的遗传组织,鉴定了三个推定的启动子,P_(RS28250),P_(RS09985)和P_(RS24685)。通过使用逆转录酶定量PCR(RT-QPCR)比较它们的表达水平来评估它们的启动子活性。我们发现RS28250,RS09985和RS24685的转录水平分别比HSPB2,编码6-羟基-3-琥珀酰吡啶羟基羟化酶的16.8,2.6和1.6倍。因此,选择两个强内源性启动子,即P_(RS28250)和P_(RS09985)以取代NIC2基因簇的原始启动子。内源性异位启动子的效果也与靶基因簇的位置有关。当启动子P_(RS28250)取代Hspb2的启动子时,所得突变体QΔAbs-δp_(hspb2):: p_(rs28250)表现出比JY-Q的尼古丁降低效率为69%。本研究表明,通过去除抑制调节蛋白并用强大的内源异位启动子取代靶促进剂来增强菌株的可行策略。分析本研究评估了同源NICR2A和NICR2B和内源异位强促进剂对尼古丁的差异效应Pseudomonas sp中的新陈代谢。菌株JY-Q。基于我们的差异分析,通过去除抑制调节蛋白NiCR2A和NiCR2B并用强源性异位启动子取代靶促进剂来提出一种可行的策略来改变野生型(WT)菌株JY-Q。所得突变体表现出尼古丁的高耐受性和降解。这些发现应该有利于通过基因组改性改善天然菌株的污染物降解能力。

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