Preparation of plasmid DNA reference material for polymyxin antibiotics resistance encoding gene detection

CHEN Jin; SU Xiumin; YANG Jing; CAO Yanwei; TIAN Yuanyuan; FENG Chengqian; ZHAO Hongyang; LU Xing’an; CUI Shenghui; YANG Baowei

doi:10.13590/j.cjfh.2022.02.003

Zhongguo shipin weisheng zazhi (Mar 2022)

Preparation of plasmid DNA reference material for polymyxin antibiotics resistance encoding gene detection

CHEN Jin,
SU Xiumin,
YANG Jing,
CAO Yanwei,
TIAN Yuanyuan,
FENG Chengqian,
ZHAO Hongyang,
LU Xing’an,
CUI Shenghui,
YANG Baowei

Affiliations

CHEN Jin: College of Food Science and Engineering， Northwest A&F University， Shaanxi Yangling 712100， China
SU Xiumin: College of Food Science and Engineering， Northwest A&F University， Shaanxi Yangling 712100， China
YANG Jing: Yangling Quality and Technical Inspection Institute， Shaanxi Yangling 712100， China
CAO Yanwei: Hebei Forest， Grass and Flower Quality Inspection and Testing Center， Hebei Shijiazhuang 050081， China
TIAN Yuanyuan: College of Food Science and Engineering， Northwest A&F University， Shaanxi Yangling 712100， China
FENG Chengqian: Market Supervision and Administration Bureau of Hantai District of Hanzhong， Shaanxi Hanzhong 723000， China
ZHAO Hongyang: Chinese Academy of Inspection and Quarantine， Beijing 100176， China
LU Xing’an: Chinese Academy of Inspection and Quarantine， Beijing 100176， China
CUI Shenghui: National Institutes for Food and Drug Control， Beijing 100500， China
YANG Baowei: College of Food Science and Engineering， Northwest A&F University， Shaanxi Yangling 712100， China

DOI: https://doi.org/10.13590/j.cjfh.2022.02.003
Journal volume & issue: Vol. 34, no. 2
pp. 203 – 210

Abstract

Read online

ObjectiveTo develop plasmid DNA reference materials that can be used for polymyxin antibiotic resistance encoding genes rapid detection.MethodsThe reference sequence of mcr1， mcr3 and mcr5 were retrieved from the National Center for Biotechnology Information to construct recombinant plasmids and strains. The recombinant strains were subcultured for 15 generations to detect the genetic stability of the target gene. The recombinant plasmid was extracted and vacuum dried to prepare the standard sample. The limit of detection （LOD） of PCR and RTqPCR was determined after the standard sample was hydrated and continuously diluted with 10fold gradient， respectively. Multitube plasmid DNA standard samples were randomly selected to qualitatively and quantitatively evaluate the uniformity and storage stability at 4 ℃， 37 ℃ and -20 ℃ by PCR and UV spectrophotometer.ResultsFragments of mcr1， mcr3 and mcr5 that encoding polymyxin resistance mechanism were successfully obtained. Target genes in the recombinant strains could stably inherited after subcultured for 15 generations. The LOD of PCR and RTqPCR of mcr1， mcr3 and mcr5 standard samples were 1.67×104 and 1.67 copies/μL， 1.31×104 and 13.1 copies/μL， 1.55×105 and 1.55 copies/μL， respectively. The mass F values of 12 standard samples randomly selected for each gene were all less than the F critical value， each gene could be detected by RTqPCR and indicating that the uniformity of the samples met the requirements. When standard samples were stored at 4 ℃ for 90 d， 37 ℃ for 14 d and -20 ℃ for 360 d， the qualitative and quantitative test result showed it was stable without significant difference.ConclusionIn this study， plasmid DNA standard samples that carrying mcr1， mcr3 and mcr5 were prepared. The target genes could be stably inherited， the standard samples had good uniformity and storage stability， and could be used as a quality control samples for polymyxin antibiotics resistance encoding genes detection and mechanisms prediction.

Published in Zhongguo shipin weisheng zazhi

ISSN: 1004-8456 (Print)
Publisher: The Editorial Office of Chinese Journal of Food Hygiene
Country of publisher: China
LCC subjects: Technology: Chemical technology: Food processing and manufacture; Technology: Home economics: Nutrition. Foods and food supply
Website: http://www.zgspws.com/zgspwszzen/home

About the journal

Abstract

Keywords