Digital PCR Validation for Characterization of Quantitative Reference Material of O157 Genomic DNA

Overview

Journal Methods Protoc

Specialty General Medicine

Date 2024 Nov 25

PMID 39584987

Authors

Claudia Patricia Tere-Pena

Martha Nancy Calderon-Ozuna

John Emerson Leguizamon Guerrero

Affiliations

Soon will be listed here.

Abstract

, a Shiga-toxin-producing (STEC), is an important pathogen related to foodborne disease that is responsible for a growing number of outbreaks worldwide and has been detected in processed meats, dairy, and fresh vegetables. Although culturing is the gold standard method for detection of this bacterium, molecular methods based on nucleic acid amplification techniques such as PCR are becoming more common because of their rapidity, sensitivity, and specificity. However, to ensure reliable results among the several alternative PCR protocols (e.g., commercial kits and reference methods), different measurement assurance tools, including validated methods, reference materials, and proficiency tests, among others, are required. Herein, we present a digital PCR method validation for detection and quantification using seven specific gene sequences; this method quantified nucleic acids from different serotypes, with a detection range of 6.6 to 7900 copies/µL and a repeatability standard deviation over the concentration range of 1% to 13.6%. The relative standard uncertainty was 3.5-14.6%, and the detection limit was 0.27 copies/µL. Subsequently, two batches of a candidate reference material based on O157:H7 genomic DNA were then produced and characterized for evaluation of copy number concentration with the validated ddPCR method, with assigned values of 164,770 ± 9251 and 172 ± 9 copies/μL. Thus, this study demonstrated the development of a validated method and reference material for dPCR and qPCR detection of O157:H7, a key STEC responsible for food poisoning.

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