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采用 60 -mer 寡核苷酸微阵列对不同污染生态系统中的生物降解和细菌 16S rRNA 基因进行分析。

Profiling of biodegradation and bacterial 16S rRNA genes in diverse contaminated ecosystems using 60-mer oligonucleotide microarray.

机构信息

Environmental Biotechnology Division, Indian Institute of Toxicology Research, Mahatma Gandhi Marg, Lucknow, Uttar Pradesh, India.

出版信息

Appl Microbiol Biotechnol. 2011 Jun;90(5):1739-54. doi: 10.1007/s00253-011-3268-5. Epub 2011 Apr 19.

Abstract

We have developed an oligonucleotide microarray for the detection of biodegradative genes and bacterial diversity and tested it in five contaminated ecosystems. The array has 60-mer oligonucleotide probes comprising 14,327 unique probes derived from 1,057 biodegradative genes and 880 probes representing 110 phylogenetic genes from diverse bacterial communities, and we named it as BiodegPhyloChip. The biodegradative genes are involved in the transformation of 133 chemical pollutants. Validation of the microarray for its sensitivity specificity and quantitation were performed using DNA isolated from well-characterized mixed bacterial cultures also having non-target strains, pure degrader strains, and environmental DNA. Application of the developed array using DNA extracted from five different contaminated sites led to the detection of 186 genes, including 26 genes unique to the individual sites. Hybridization of 16S rRNA probes revealed the presence of bacteria similar to well-characterized genera involved in biodegradation of various pollutants. Genes involved in complete degradation pathways for hexachlorocyclohexane (lin), 1,2,4-trichlorobenzene (tcb), naphthalene (nah), phenol (mph), biphenyl (bph), benzene (ben), toluene (tbm), xylene (xyl), phthalate (pht), Salicylate (sal), and resistance to mercury (mer) were detected with highest intensity. The most abundant genes belonged to the enzyme hydroxylases, monooxygenases, and dehydrogenases which were present in all the five samples. Thus, the array developed and validated here shall be useful in assessing not only the biodegradative potential but also the composition of environmentally useful bacteria, simultaneously, from hazardous ecosystems.

摘要

我们开发了一种寡核苷酸微阵列,用于检测生物降解基因和细菌多样性,并在五个污染生态系统中进行了测试。该阵列具有 60 -mer 寡核苷酸探针,由 1057 种生物降解基因中的 14327 个独特探针和来自不同细菌群落的 880 个代表 110 个系统发育基因的探针组成,我们将其命名为 BiodegPhyloChip。这些生物降解基因参与了 133 种化学污染物的转化。使用从具有非目标菌株、纯降解菌株和环境 DNA 的特征良好的混合细菌培养物中分离的 DNA 对微阵列的灵敏度、特异性和定量进行了验证。使用从五个不同污染地点提取的 DNA 应用开发的阵列导致检测到 186 个基因,包括 26 个特定于各个地点的基因。16S rRNA 探针的杂交揭示了存在与各种污染物生物降解有关的特征良好的细菌。涉及六氯环己烷(Lin)、1,2,4-三氯苯(Tcb)、萘(Nah)、苯酚(Mph)、联苯(Bph)、苯(Ben)、甲苯(Tbm)、二甲苯(Xyl)、邻苯二甲酸酯(Pht)、水杨酸(Sal)和汞抗性(Mer)的完整降解途径的基因的检测强度最高。最丰富的基因属于所有五个样本中都存在的酶羟基化酶、单加氧酶和脱氢酶。因此,这里开发和验证的阵列不仅将有助于评估生物降解潜力,而且还将有助于同时评估有害生态系统中有用的环境细菌的组成。

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