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| DOI | 10.1016/j.mimet.2018.07.005 |
| Quantification of plasmid DNA standards for US EPA fecal indicator bacteria qPCR methods by droplet digital PCR analysis | |
| Sivaganesan, Mano1; Varma, Manju2; Siefring, Shawn2; Haugland, Richard2 | |
| 发表日期 | 2018-09-01 |
| ISSN | 0167-7012 |
| 卷号 | 152页码:135-142 |
| 英文摘要 | An obstacle to establishing widely useful data acceptance criteria for U.S. Environmental Protection Agency (EPA) qPCR methods has been the unavailability of standardized reference materials. Earlier versions of EPA Methods 1609 and 1611 for enterococci used cellular reference materials for quantifying enterococci in unknown test samples, however, EPA updates to these fundamentally DNA-based analysis methods have shifted toward the use of DNA standards. This report describes the application of droplet digital PCR (ddPCR) analysis for the quantification of a set of synthetic plasmid DNA standards that have been made available for updated EPA Methods 1609.1 and 1611.1 as well as for EPA Draft Method C for Escherichia coli. To obtain the most accurate concentration estimates possible, part of this effort was to develop a data analysis model for determining the fluorescence thresholds that distinguish positive from negative droplets produced by the ddPCR reactions. Versions of this model are described for applications with individual reactions, multiple reactions within a ddPCR system run, and multiple reactions within and across different system runs. The latter version was applied toward determinations of error in the concentration estimates of the standards from replicate analyses of each standard in multiple ddPCR system runs. Mean concentration estimates for the five standards from the ddPCR analyses were 4.356, 3.381, 2.371, 1.641 and 1.071 log(10) copies/5 mu L with associated standard deviations of 0.074, 0.082, 0.108, 0.131 and 0.188, respectively. These estimates contrasted with expected log(10) concentrations of 4.6, 3.6, 2.6, 1.9 and 1.3 copies/5 mu L, respectively, based on the yield of the plasmid reported by the vendor and spectrophotometric analysis of the initial stock solution of this material. These results illustrate how the analyses of original stocks may lead to potential bias(es) in the concentration estimates of final DNA standards and subsequently in the estimates of unknown test samples determined from these standards in qPCR analyses. |
| 英文关键词 | QPCR;DNA standards;EPA Methods 1609.1 and 1611.1;Digital droplet PCR |
| 语种 | 英语 |
| WOS记录号 | WOS:000447113600022 |
| 来源期刊 | JOURNAL OF MICROBIOLOGICAL METHODS
 |
| 来源机构 | 美国环保署 |
| 文献类型 | 期刊论文 |
| 条目标识符 | http://gcip.llas.ac.cn/handle/2XKMVOVA/59447 |
| 作者单位 | 1.US EPA, Off Res & Dev, Natl Risk Management Res Lab, 26 WML King Dr, Cincinnati, OH 45268 USA; 2.US EPA, Off Res & Dev, Natl Exposure Res Lab, 26 WML King Dr, Cincinnati, OH 45268 USA |
| 推荐引用方式 GB/T 7714 | Sivaganesan, Mano,Varma, Manju,Siefring, Shawn,et al. Quantification of plasmid DNA standards for US EPA fecal indicator bacteria qPCR methods by droplet digital PCR analysis[J]. 美国环保署,2018,152:135-142. |
| APA | Sivaganesan, Mano,Varma, Manju,Siefring, Shawn,&Haugland, Richard.(2018).Quantification of plasmid DNA standards for US EPA fecal indicator bacteria qPCR methods by droplet digital PCR analysis.JOURNAL OF MICROBIOLOGICAL METHODS,152,135-142. |
| MLA | Sivaganesan, Mano,et al."Quantification of plasmid DNA standards for US EPA fecal indicator bacteria qPCR methods by droplet digital PCR analysis".JOURNAL OF MICROBIOLOGICAL METHODS 152(2018):135-142. |
| 条目包含的文件 | 条目无相关文件。 | |||||
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