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利用功能基因分析对生物反应器中苯酚羟化酶多样性进行定量评估。

Quantitative assessment of phenol hydroxylase diversity in bioreactors using a functional gene analysis.

作者信息

Basile Laura A, Erijman Leonardo

机构信息

Instituto de Investigaciones en Ingeniería Genética y Biología Molecular (INGEBI-CONICET), Vuelta de Obligado 2490, ADN1428 Buenos Aires, Argentina.

出版信息

Appl Microbiol Biotechnol. 2008 Apr;78(5):863-72. doi: 10.1007/s00253-008-1351-3. Epub 2008 Jan 17.

Abstract

We describe a quantitative analysis of the genetic diversity of phenol-degrading potential in bacterial communities from laboratory-scale activated sludge. Genomic DNA extracted from activated sludge from two sequential batch reactors fed with synthetic sewage plus phenol was amplified using conserved primers for the major subunit of the phenol hydroxylase (LmPH) gene and used to generate clone libraries. Following phylogenetic analysis, 59 sequences containing a 470-bp fragment clustered into six distinct subgroups with a genetic distance of 8%, most likely representing ecologically relevant variants of the enzyme. Seven sets of primers were designed to target the six clusters and used to obtain quantitative information on the dynamics of LmPH gene diversity using real-time PCR assays throughout 9 months of bioreactors operation. Total LmPH gene copy number remained approximately steady in phenol-amended and control reactors. However, a significant increase in phenol-degrading activity in the phenol-amended sludge was accompanied by a parallel increase in LmPH gene diversity, suggesting that phenol degradation in the activated sludge depends on the combined activity of a number of redundant species.

摘要

我们描述了对实验室规模活性污泥中细菌群落苯酚降解潜力的遗传多样性进行的定量分析。从两个连续批次反应器中以合成污水加苯酚为进料的活性污泥中提取的基因组DNA,使用针对苯酚羟化酶(LmPH)基因主要亚基的保守引物进行扩增,并用于构建克隆文库。经过系统发育分析,59个包含470 bp片段的序列聚为6个不同的亚组,遗传距离为8%,很可能代表该酶的生态相关变体。设计了7组引物靶向这6个簇,并用于通过实时PCR测定在生物反应器运行的9个月中获取关于LmPH基因多样性动态的定量信息。在添加苯酚的反应器和对照反应器中,LmPH基因的总拷贝数大致保持稳定。然而,添加苯酚的污泥中苯酚降解活性的显著增加伴随着LmPH基因多样性的平行增加,这表明活性污泥中的苯酚降解取决于多种冗余物种的联合活性。

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