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Development of a 16S rRNA gene sequence as a biomarker specific to the gastrointestinal tract and feces of swine based on suppressive subtractive hybridization.

机译:基于抑制性消减杂交技术开发了一种16S rRNA基因序列,作为猪胃肠道和粪便的生物标记物。

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摘要

Fecal contamination of water bodies causes environmental issues and human health risks. Swine are a major contributor of fecal inputs to environmental waters due to their importance in American agriculture. Water quality currently is regulated using fecal coliforms, which have natural reservoirs in the environment and may not correlate with pathogens. In recent years there has been a shift towards microbial source tracking (MST). MST employs microbiological, genotypic, phenotypic and chemical methods to determine the source of fecal pollution in water bodies. Previous studies aimed at developing swine fecal biomarkers have had limited success. The overall objective of this research was to identify a microbial marker for swine fecal contamination. Swine (n=8) and non-target fecal samples (n=23) were collected in Morgantown, WV and the surrounding area. Additional soil (n=2) and lagoon (n=3) samples impacted with swine manure and soil (n=3) samples from areas not expected to be impacted by swine manure were collected. DNA extraction was performed followed by 16S rRNA amplification. The amplified DNA was taken into suppressive subtractive hybridization (SSH) to enrich for swine specific sequences. The final products obtained in SSH were cloned and sequenced. Swine-specific primers were designed and tested in PCR and qPCR assays against swine and non-target DNA. Sequence A5, closely related to Prevotellaceae, was detected in all swine samples tested, as well as the environmental samples impacted by swine manure. The relationship between closely related 16S rRNA sequences of Prevotellaceae and the swine marker were compared in a phylogenetic tree. The SYBR green qPCR assay did show amplification of sequences in cattle, human, and two non-target soil samples; however, apparent positive detection of the swine marker was rejected based on dissociation profiles. Therefore, the SYBR green qPCR assay was determined to be specific to detect the swine marker in target samples and environmental samples impacted by swine manure and to discriminate between closely related genes in non-target fecal material. Furthermore, the results of this study provide evidence that SSH is an effective tool to generate source-specific markers. Future efforts will increase the sensitivity of the qPCR assay.
机译:粪便污染水体会导致环境问题和人类健康风险。由于猪在美国农业中的重要性,因此是粪便对环境水投入的主要贡献者。目前,粪便中的大肠菌群可调节水质,大肠菌群在环境中具有天然的储水库,可能与病原体无关。近年来,已经向微生物源跟踪(MST)转移。 MST采用微生物学,基因型,表型和化学方法来确定水体中粪便污染的来源。先前旨在开发猪粪便生物标志物的研究成果有限。这项研究的总体目标是确定猪粪便污染的微生物标记。在Morgantown,WV和周边地区收集了猪(n = 8)和非目标粪便样本(n = 23)。收集了另外受猪粪影响的土壤(n = 2)和泻湖(n = 3)样本,以及预期未受猪粪影响的地区的土壤(n = 3)样本。进行DNA提取,然后进行16S rRNA扩增。将扩增的DNA用于抑制性消减杂交(SSH),以丰富猪的特定序列。克隆并测序了在SSH中获得的最终产物。设计猪特异性引物并在针对猪和非靶DNA的PCR和qPCR分析中进行测试。在所有测试的猪样品以及受猪粪影响的环境样品中均检测到与前鞭毛科密切相关的序列A5。在系统发育树中比较了近邻Prepretellaceae的16S rRNA序列与猪标记之间的关系。 SYBR green qPCR测定法确实显示了牛,人和两个非目标土壤样品中的序列扩增。然而,基于解离曲线,猪标志物的明显阳性检测被拒绝。因此,SYBR green qPCR测定被确定为特异性检测受猪粪影响的目标样品和环境样品中的猪标志物,并能区分非目标粪便中密切相关的基因。此外,这项研究的结果提供了证据,证明SSH是生成特定来源标记的有效工具。未来的努力将提高qPCR分析的灵敏度。

著录项

  • 作者

    Sayre, Autumn.;

  • 作者单位

    West Virginia University.;

  • 授予单位 West Virginia University.;
  • 学科 Biology Microbiology.
  • 学位 M.S.
  • 年度 2013
  • 页码 67 p.
  • 总页数 67
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

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