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建立定量 PCR 方法以定量检测淡水系统中的产土腥素潜能和鱼腥藻。

Establishment of quantitative PCR methods for the quantification of geosmin-producing potential and Anabaena sp. in freshwater systems.

机构信息

State Key Laboratory of Environmental Aquatic Chemistry, Research Center for Eco-Environmental Sciences, Chinese Academy of Sciences, 18 Shuangqing Rd., Haidian, Beijing 100085, China.

出版信息

Water Res. 2013 Jun 15;47(10):3444-54. doi: 10.1016/j.watres.2013.03.043. Epub 2013 Apr 6.

DOI:10.1016/j.watres.2013.03.043
PMID:23622984
Abstract

Geosmin has often been associated with off-flavor problems in drinking water with Anabaena sp. as the major producer. Rapid on-site detection of geosmin-producers as well as geosmin is important for a timely management response to potential off-flavor events. In this study, quantitative polymerase chain reaction (qPCR) methods were developed to detect the levels of Anabaena sp. and geosmin, respectively, by designing two PCR primer sets to quantify the rpoC1 gene (ARG) and geosmin synthase one (GSG) in Anabaena sp. in freshwater systems. The ARG density determined by qPCR assay is highly related to microscopic cell count (r(2) = 0.726, p < 0.001), and the limit of detection (LOD) and limit of quantification (LOQ) of the qPCR method were 0.02 pg and 0.2 pg of DNA, respectively. At the same time, the relationship between geosmin concentrations measured by gas chromatography-mass spectrometry (GC-MS) and GSG copies was also established (r(2) = 0.742, p < 0.001) with similar LOD and LOQ values. Using the two qPCR protocols, we succeeded in measuring different levels of ARG and GSG copies in different freshwater systems with high incidence environmental substrata and diverse ecological conditions, showing that the methods developed could be applied for environmental monitoring. Moreover, comparing to the microscopic count and GC-MS analytical methods, the qPCR methods can reduce the time-to-results from several days to a few hours and require considerably less traditional algal identification and taxonomic expertise.

摘要

鱼腥藻常常与饮用水中的异味问题有关,是主要的产生者。快速现场检测鱼腥藻和土臭素对于及时管理潜在异味事件非常重要。在这项研究中,通过设计两个 PCR 引物对,分别定量淡水系统中鱼腥藻的 rpoC1 基因(ARG)和土臭素合酶基因(GSG),开发了定量聚合酶链反应(qPCR)方法来分别检测鱼腥藻和土臭素的水平。qPCR 测定的 ARG 密度与显微镜细胞计数高度相关(r²=0.726,p<0.001),qPCR 方法的检测限(LOD)和定量限(LOQ)分别为 0.02pg 和 0.2pg DNA。同时,还建立了气相色谱-质谱(GC-MS)测定的土臭素浓度与 GSG 拷贝数之间的关系(r²=0.742,p<0.001),具有相似的 LOD 和 LOQ 值。使用这两种 qPCR 方案,我们成功地测量了不同淡水系统中不同水平的 ARG 和 GSG 拷贝数,这些系统具有高发生率的环境基质和多样的生态条件,表明所开发的方法可用于环境监测。此外,与显微镜计数和 GC-MS 分析方法相比,qPCR 方法可以将结果时间从几天缩短到几个小时,并且需要相当少的传统藻类鉴定和分类专业知识。

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