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基于快速定量 PCR 与传统培养法对娱乐用水中肠球菌属和大肠杆菌计数的比较。

Comparison of rapid quantitative PCR-based and conventional culture-based methods for enumeration of Enterococcus spp. and Escherichia coli in recreational waters.

机构信息

Institute of Marine Sciences, University of North Carolina at Chapel Hill, Morehead City, NC 28557, USA.

出版信息

Appl Environ Microbiol. 2010 Nov;76(22):7437-43. doi: 10.1128/AEM.00651-10. Epub 2010 Sep 24.

Abstract

Recreational water quality is currently monitored using culture-based methods that require 18 to 96 h for results. Quantitative PCR (QPCR) methods that can be completed in less than 2 h have been developed, but they could yield different results than the conventional methods. We present two studies in which samples were processed simultaneously for Enterococcus spp. and Escherichia coli using two culture-based methods (EPA method 1600 and Enterolert/Colilert-18) and QPCR. The proprietary QPCR assays targeted the 23S rRNA (Enterococcus spp.) and uidA (E. coli) genes and were conducted using lyophilized beads containing all reagents. In the first study, the QPCR method developers processed 54 blind samples that were inoculated with sewage or pure cultures or were ambient beach samples. The second study involved 163 samples processed by water quality personnel. The correlation between results of QPCR and EPA 1600 during the first study (r²) was 0.69 for Enterococcus spp., which was less than that observed between the culture-based methods (r², 0.87). During the second study, the correlations were similar. No false positives occurred in either study when QPCR-based assays were used with blank samples. Levels of reproducibility measured through coefficients of variation were similar for results by Enterococcus QPCR and culture-based methods during both studies but were higher for E. coli QPCR results in the first study. Regarding the concentration at which beach management decisions are issued in the State of California, the agreement between results of Enterococcus QPCR and EPA method 1600 was 88%, compared to 94% agreement between EPA method 1600 and Enterolert. The beach management decision agreement between E. coli QPCR and Colilert-18 was 94%. The samples showing disagreement suggested an underestimation bias for QPCR.

摘要

休闲用水水质目前采用基于培养的方法进行监测,结果需要 18 至 96 小时。现已开发出可在 2 小时内完成的定量 PCR(QPCR)方法,但它们的结果可能与传统方法不同。我们展示了两项研究,其中同时使用两种基于培养的方法(EPA 方法 1600 和 Enterolert/Colilert-18)和 QPCR 对粪肠球菌和大肠杆菌进行处理,同时对样本进行处理。专有的 QPCR 检测针对 23S rRNA(粪肠球菌)和 uidA(大肠杆菌)基因,并使用含有所有试剂的冻干珠进行检测。在第一项研究中,QPCR 方法的开发者处理了 54 个盲样,这些盲样接种了污水或纯培养物或环境海滩样本。第二项研究涉及由水质人员处理的 163 个样本。第一项研究中 QPCR 方法与 EPA 1600 之间的相关性(r²)为 0.69,低于基于培养的方法之间的相关性(r²,0.87)。在第二项研究中,相关性相似。在两个研究中,使用空白样本进行基于 QPCR 的检测时,均未出现假阳性。在两个研究中,粪肠球菌 QPCR 和基于培养的方法的重复性测量结果的变异系数相似,但第一个研究中大肠杆菌 QPCR 结果的变异系数更高。在加利福尼亚州,针对海滩管理决策的浓度,粪肠球菌 QPCR 与 EPA 方法 1600 的结果一致性为 88%,而 EPA 方法 1600 与 Enterolert 的一致性为 94%。E. coli QPCR 与 Colilert-18 之间的海滩管理决策一致性为 94%。显示不一致的样本表明 QPCR 存在低估偏差。

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