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Microdiversity of phenol hydroxylase genes among phenol-degrading isolates of Alcaligenes sp. from an activated sludge system

机译:Alcaligenes sp。的苯酚降解菌中酚羟化酶基因的多样性。来自活性污泥系统

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摘要

Enterobacterial repetitive intergenic consensus (ERIC)-PCR fingerprinting classified 97 phenol-degrading isolates with identical amplified ribosomal DNA restriction analysis (ARDRA) patterns into six genotypic groups. The 16S rRNA gene of the representative isolate of each group had higher than 99.47% common identity with each other and higher than 98% identity with the type strain of Alcaligenes faecalis. PCR-TGGE (temperature gradient gel electrophoresis) analysis of the genes of the largest subunit of the multi-component phenol hydroxylase (LmPH) in each isolate followed with sequencing showed that isolates within each ERIC-PCR group had identical LmPH gene sequences. Among the six different ERIC-PCR groups, two were found to harbor two different LmPH genes encoding low- and high-Ks (affinity constants) phenol hydroxylases, and the low-Ks type LmPH was identical in sequence with one predominant LmPH of the parental activated sludge. Three ERIC-PCR groups had only the high-Ks type and one had no sequence similar to the known LmPHs. Our work suggests that there is no correlation between the phylogenetic groupings of phenol-degrading bacteria and their LmPH genotypes possibly due to extensive horizontal gene transfer of this functional gene.
机译:肠杆菌重复基因间共有(ERIC)-PCR指纹图谱将具有相同扩增核糖体DNA限制分析(ARDRA)模式的97种苯酚降解菌株分为六个基因型组。每组代表性分离株的16S rRNA基因彼此之间的同源性均高于99.47%,与粪便产碱杆菌的类型株具有高于98%的同一性。对每个分离物中的多组分酚羟化酶(LmPH)最大亚基的基因进行PCR-TGGE(温度梯度凝胶电泳)分析,然后测序,结果表明,每个ERIC-PCR组中的分离物具有相同的LmPH基因序列。在六个不同的ERIC-PCR组中,发现其中两个具有两个编码低Ks和高Ks(亲和常数)酚羟化酶的LmPH基因,并且低Ks型LmPH与亲本中的一个主要LmPH序列相同活性污泥。三个ERIC-PCR组只有高Ks型,一个没有类似于已知LmPHs的序列。我们的工作表明,苯酚降解细菌的系统发育组与其LmPH基因型之间没有相关性,这可能是由于该功能基因的广泛水平基因转移所致。

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