Establishment of a qPCR method to detect Staphylococcus xylosus and its application
10.3969/j.issn.1005-4847.2024.01.010
- VernacularTitle:木糖葡萄球菌实时荧光定量PCR检测方法的建立及其应用
- Author:
Lingzhi YU
1
;
Liping FENG
;
Zhihao KONG
;
Qi ZHU
;
Xiaofeng WEI
Author Information
1. 上海实验动物研究中心,上海 201203
- Keywords:
Staphylococcus xylosus;
detection method;
qPCR
- From:
Acta Laboratorium Animalis Scientia Sinica
2024;32(1):73-79
- CountryChina
- Language:Chinese
-
Abstract:
Objective To establish and evaluate a method for rapid and sensitive S.xylosus detection using qPCR(real-time quantitative PCR).Methods A gehM gene fragment was selected as the target for S.xylosus.A set of specific primers was synthesized and a qPCR method was established to detect S.xylosus.A S.xylosus standard strain and other non-target strains were chosen for analysis.DNA of S.xylosus was diluted 10-fold to determine its sensitivity.Clinical samples were tested,and positive products were sequenced.The result were compared with those of bacterial culture.Results S.xylosus had a specific amplification curve,whereas other non-S.xylosus species did not,indicating that the primers were specific for S.xylosus.Sensitivity was 100 fg/μL DNA.Repeatability within and between groups was less than 3%.A total of 60 clinical samples were analyzed,of which five samples had a typical S curve.qPCR products were sequenced and BLAST searched.The similarity of the gene sequences was 99.63%,indicating that the sample was positive for the S.xylosus gehM gene with a positivity rate of 8.3%.However,the positivity rate of bacterial culture was 6.7%.The positivity rate of qPCR was slightly higher than that of the culture.Conclusions The established qPCR method is rapid with high sensitivity and specificity,and can be used to detect S.xylosus.
