Evaluation of microbial qPCR workflows using engineered Saccharomyces cerevisiae

Q1 Biochemistry, Genetics and Molecular Biology

Biomolecular Detection and Quantification Pub Date : 2016-03-01 DOI:10.1016/j.bdq.2016.01.001

S.M. Da Silva , L.K. Vang , N.D. Olson , S.P. Lund , A.S. Downey , Z. Kelman , M.L. Salit , N.J. Lin , J.B. Morrow

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引用次数: 3

Abstract

Aims

We describe the development and interlaboratory study of modified Saccharomyces cerevisiae as a candidate material to evaluate a full detection workflow including DNA extraction and quantitative polymerase chain reaction (qPCR).

Methods and results

S. cerevisiae NE095 was prepared by stable insertion of DNA sequence External RNA Control Consortium-00095 into S. cerevisiae BY4739 to convey selectivity. For the interlaboratory study, a binomial regression model was used to select three cell concentrations, high (4 × 10⁷ cells ml⁻¹), intermediate (4 × 10⁵ cells ml⁻¹) and low (4 × 10³ cells ml⁻¹), and the number of samples per concentration. Seven participants, including potential end users, had combined rates of positive qPCR detection (quantification cycle <37) of 100%, 40%, and 0% for high, intermediate, and low concentrations, respectively.

Conclusions

The NE095 strain was successfully detected by all participants, with the high concentration indicating a potential target concentration for a reference material.

Significance and impact of the study

The engineered yeast has potential to support measurement assurance for the analytical process of qPCR, encompassing the method, equipment, and operator, to increase confidence in results and better inform decision-making in areas of applied microbiology. This material can also support process assessment for other DNA-based detection technologies.

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利用工程酿酒酵母评价微生物qPCR工作流程

我们描述了修饰酿酒酵母的发展和实验室间研究，作为评估完整检测工作流程的候选材料，包括DNA提取和定量聚合酶链反应(qPCR)。方法与结果。将DNA序列External RNA Control Consortium-00095稳定插入酿酒酵母BY4739中以传递选择性，制备出酿酒酵母NE095。对于实验室间研究，使用二项回归模型选择三种细胞浓度，高(4 × 107细胞ml - 1)，中等(4 × 105细胞ml - 1)和低(4 × 103细胞ml - 1)，以及每个浓度的样品数量。7名参与者，包括潜在的最终用户，在高、中、低浓度下qPCR检测阳性率分别为100%、40%和0%(定量周期为37)。结论NE095菌株被所有参与者成功检出，该菌株的浓度较高，可能是标准物质的目标浓度。研究的意义和影响工程酵母有潜力支持qPCR分析过程的测量保证，包括方法、设备和操作人员，以增加对结果的信心，并更好地为应用微生物学领域的决策提供信息。该材料还可以支持其他基于dna的检测技术的工艺评估。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Biomolecular Detection and Quantification Biochemistry, Genetics and Molecular Biology-Biochemistry

CiteScore

14.20

自引率

0.00%

发文量

审稿时长

8 weeks