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Specific and effective detection of anammox bacteria using PCR primers targeting the 16S rRNA gene and functional genes

机译:使用PCR引物靶向16S rRNA基因和功能基因的特异性和有效检测厌氧菌细菌

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摘要

Anaerobic ammonium-oxidizing (anammox) bacteria play an important role in the nitrogen cycle by coupling ammonium and nitrite to produce dinitrogen gas (N_2). Polymerase chain reaction (PCR) is a fast, simple, and sensitive method that is widely used to assess the diversity, abundance, and activity of the slow-growing bacteria. In this review, we summarize and evaluate the wide variety of PCR primers targeting the 16S rRNA gene and functional genes (hzo, nir, and hzs) of anammox bacteria for their effectiveness and efficiencies in detecting this group of bacteria in different sample types. Furthermore, the efficiencies of different universal high-throughput sequencing 16S rRNA gene primers in anammox bacteria investigations were also evaluated to provide a reference for primer selection. Based on our in silica evaluation results, none of the 16S rRNA gene primers could recover all of the known anammox bacteria, but multiple hzo and hzs gene primers could accomplish this task. However, uncertain copies (1-3 copies) of hzo genes were identified in the genomes, and the hydrazine oxidation reaction catalyzed by hydrazine oxidoreductases (HZOs) can also be catalyzed by other hydroxylamine oxidoreductases (HAOs) in anammox bacteria, which can potentially result in large deviations in hzo-based qPCR and RT-qPCR analyses and results. Therefore, the use of optimal primers targeting unique hzs genes are recommended, although the efficiencies of these newly designed primers need further verification in practical applications. This article provides comprehensive information for the effective and specific detection of anammox bacteria using specific primers targeting the 16S rRNA gene and functional genes and serves as a basis for future high-quality primer design.
机译:厌氧铵氧化(厌氧毒素)细菌通过偶联铵和亚硝酸盐产生二氮气(N_2)在氮循环中发挥着重要作用。聚合酶链反应(PCR)是一种快速,简单,敏感的方法,广泛用于评估缓慢生长细菌的多样性,丰度和活性。在本次综述中,我们总结和评估了靶向16S rRNA基因和功能基因(HZO,NIR和HZS)的各种PCR引物,用于厌氧细菌的有效性和效率检测不同样品类型的细菌。此外,还评价了不同通用的高通量测序16S rRNA基因引物的效率,以提供引物选择的参考。基于我们的二氧化硅评估结果,16S rRNA基因引物中没有一个可以恢复所有已知的厌氧菌细菌,但多个HZO和HZS基因引物可以实现这项任务。然而,在基因组中鉴定了不确定的拷贝(1-3份)的HZO基因,并且含有肼氧化还原酶(HZOS)催化的肼氧化反应也可以通过厌氧细菌的其它羟胺氧化酶(HAOS)催化,这可能会导致基于HZO的QPCR和RT-QPCR分析和结果的大偏差。因此,建议使用靶向独特的HzS基因的最佳引物,尽管这些新设计的引物的效率需要进一步验证实际应用。本文提供了使用靶向16S rRNA基因和功能基因的特异性引物的有效和特异性检测的综合信息,并用作未来高质量底漆设计的基础。

著录项

  • 来源
    《The Science of the Total Environment》 |2020年第10期|139387.1-139387.12|共12页
  • 作者单位

    Laboratory of Environmental Microbiology and Toxicology School of Biological Sciences The University of Hong Kong Pokfulam Road Hong Kong SAR Hong Kong People's Republic of China Environmental Engineering Guangdong Technion Israel Institute of Technology 241 Daxue Road Shantou Guangdong 515063 People's Republic of China;

    Shenzhen Key Laboratory of Marine Microbiome Engineering Institute for Advanced Study Shenzhen University Shenzhen 518060 People's Republic of China;

    School of Resource and Environmental Engineering East China University of Science and Technology 130 Meilong Road Shanghai 200237 People's Republic of China;

    Department of Civil and Environmental Engineering The University of Hong Kong Pokfulam Road Hong Kong People's Republic of China;

    Institute of Environmental Engineering National Chiao Tung University 1001 University Road Hsinchu City 30010 Taiwan;

    Department of Urban Water- and Waste Management University of Duisburg-Essen Universitatsstrasse 15 45141 Essen Germany;

    School of Food and Biotechnology Guangdong Industry Polytechnic Guangzhou Guangdong 510300 People's Republic of China Environmental Engineering Guangdong Technion Israel Institute of Technology 241 Daxue Road Shantou Guangdong 515063 People's Republic of China;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

    Anammox bacteria; PCR primer; 16S rRNA gene; Functional gene; Efficiency; Specificity;

    机译:厌氧细菌;PCR引物;16s rRNA基因;功能基因;效率;特异性;

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