[Development and preliminary application of a multiplex PCR assay for simultaneous detection of four intestinal parasites in goats].

Q3 Medicine

中国血吸虫病防治杂志 Pub Date : 2024-06-20 DOI:10.16250/j.32.1374.2024046

Y Li, X Mu, H Xu, X Luo, R Yu, X Xu, L Yang, X Yu, Y Hong

{"title":"[Development and preliminary application of a multiplex PCR assay for simultaneous detection of four intestinal parasites in goats].","authors":"Y Li, X Mu, H Xu, X Luo, R Yu, X Xu, L Yang, X Yu, Y Hong","doi":"10.16250/j.32.1374.2024046","DOIUrl":null,"url":null,"abstract":"Objective: To develop a multiplex PCR assay for simultaneous detection of four intestinal parasites, including Giardia duodenalis, Cryptosporidium parvum, Enterocytozoon bieneusi and Moniezia, and to preliminarily evaluate its detection efficiency.Methods: Four pairs of specific primers were designed based on the conserved sequences of the corresponding genes of G. duodenalis (GenBank accession number: XM_001710026.2), C. parvum (GenBank accession number: XM_626998.1), E. bieneusi (GenBank accession number: KJ719492.1) and Moniezia (GenBank accession number: OM296991.1) retrieved from the GenBank database, and a multiplex PCR assay for simultaneous detection of G. duodenalis, C. parvum, E. bieneusi and Moniezia was developed and optimized. A total of 116 fresh goat stool samples were collected from four goat farms in Zhanjiang City, Guangdong Province during the period from October to December 2022, including 96 samples used for evaluating the detection efficacy of the multiplex PCR assay, and 20 samples as baseline controls for sample testing. Genomic DNA extracted from 96 goat stool samples was tested using the single-target PCR assay and the developed multiplex PCR assay, and the sensitivity, specificity, positive predictive value, and negative predictive value of the multiplex PCR assay were evaluated for detection of G. duodenalis, C. parvum, E. bieneusi and Moniezia DNA in goat stool samples with the single-target PCR assay as the gold standard.Results: The multiplex PCR assay developed in this study allowed simultaneous amplification of specific gene fragments of G. duodenalis, C. parvum, E. bieneusi and Moniezia, with 1 400, 755, 314 bp and 585 bp in sizes, respectively, and the detection limit was 102 and higher copies of parasite DNA clones, while the multiplex PCR assay was negative for gene amplification of Schistosoma japonicum, Fasciola hepatica, Echinococcus granulosus, Blastocystis hominis and Homalogaster paloniae. Single-target PCR assay and the developed multiplex PCR assay were employed to test DNA samples extracted from 96 goat stool samples, and single-target PCR assay tested positive in 40 goat stool samples (41.67%), including 39 positive samples tested with the multiplex PCR assay, with a mean coincidence rate of 97.50% (39/40). The multiplex PCR assay tested positive for G. duodenalis DNA in 26 goat stool samples (27.10%), C. parvum DNA in 22 samples (22.90%), E. bieneusi DNA in 24 samples (25.00%), and Moniezia in 9 samples (9.40%), which was consistent with the detection using the single-target PCR assay. The sensitivity, negative predictive value, and positive predictive value of the multiplex PCR assay were 96.15%, 95.83%, 100.00% and 100.00%, 98.90%, 98.92%, 100.00% and 100.00%, 100.00%, 100.00%, 100.00% and 100.00% for detection of G. duodenalis, C. parvum, E. bieneusi and Moniezia DNA in goat stool samples, respectively, if the single-target PCR assay served as the gold standard.Conclusions: A highly sensitive and specific multiplex PCR assay has been developed for simultaneous detection of G. duodenalis, C. parvum, E. bieneusi and Moniezia in goats, which is suitable for rapid, large-scale screening of intestinal parasites in sheep stool samples.","PeriodicalId":38874,"journal":{"name":"中国血吸虫病防治杂志","volume":"36 4","pages":"376-383"},"PeriodicalIF":0.0000,"publicationDate":"2024-06-20","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"","citationCount":"0","resultStr":null,"platform":"Semanticscholar","paperid":null,"PeriodicalName":"中国血吸虫病防治杂志","FirstCategoryId":"3","ListUrlMain":"https://doi.org/10.16250/j.32.1374.2024046","RegionNum":0,"RegionCategory":null,"ArticlePicture":[],"TitleCN":null,"AbstractTextCN":null,"PMCID":null,"EPubDate":"","PubModel":"","JCR":"Q3","JCRName":"Medicine","Score":null,"Total":0}

引用次数: 0

Abstract

Objective: To develop a multiplex PCR assay for simultaneous detection of four intestinal parasites, including Giardia duodenalis, Cryptosporidium parvum, Enterocytozoon bieneusi and Moniezia, and to preliminarily evaluate its detection efficiency.

Methods: Four pairs of specific primers were designed based on the conserved sequences of the corresponding genes of G. duodenalis (GenBank accession number: XM_001710026.2), C. parvum (GenBank accession number: XM_626998.1), E. bieneusi (GenBank accession number: KJ719492.1) and Moniezia (GenBank accession number: OM296991.1) retrieved from the GenBank database, and a multiplex PCR assay for simultaneous detection of G. duodenalis, C. parvum, E. bieneusi and Moniezia was developed and optimized. A total of 116 fresh goat stool samples were collected from four goat farms in Zhanjiang City, Guangdong Province during the period from October to December 2022, including 96 samples used for evaluating the detection efficacy of the multiplex PCR assay, and 20 samples as baseline controls for sample testing. Genomic DNA extracted from 96 goat stool samples was tested using the single-target PCR assay and the developed multiplex PCR assay, and the sensitivity, specificity, positive predictive value, and negative predictive value of the multiplex PCR assay were evaluated for detection of G. duodenalis, C. parvum, E. bieneusi and Moniezia DNA in goat stool samples with the single-target PCR assay as the gold standard.

Results: The multiplex PCR assay developed in this study allowed simultaneous amplification of specific gene fragments of G. duodenalis, C. parvum, E. bieneusi and Moniezia, with 1 400, 755, 314 bp and 585 bp in sizes, respectively, and the detection limit was 10² and higher copies of parasite DNA clones, while the multiplex PCR assay was negative for gene amplification of Schistosoma japonicum, Fasciola hepatica, Echinococcus granulosus, Blastocystis hominis and Homalogaster paloniae. Single-target PCR assay and the developed multiplex PCR assay were employed to test DNA samples extracted from 96 goat stool samples, and single-target PCR assay tested positive in 40 goat stool samples (41.67%), including 39 positive samples tested with the multiplex PCR assay, with a mean coincidence rate of 97.50% (39/40). The multiplex PCR assay tested positive for G. duodenalis DNA in 26 goat stool samples (27.10%), C. parvum DNA in 22 samples (22.90%), E. bieneusi DNA in 24 samples (25.00%), and Moniezia in 9 samples (9.40%), which was consistent with the detection using the single-target PCR assay. The sensitivity, negative predictive value, and positive predictive value of the multiplex PCR assay were 96.15%, 95.83%, 100.00% and 100.00%, 98.90%, 98.92%, 100.00% and 100.00%, 100.00%, 100.00%, 100.00% and 100.00% for detection of G. duodenalis, C. parvum, E. bieneusi and Moniezia DNA in goat stool samples, respectively, if the single-target PCR assay served as the gold standard.

Conclusions: A highly sensitive and specific multiplex PCR assay has been developed for simultaneous detection of G. duodenalis, C. parvum, E. bieneusi and Moniezia in goats, which is suitable for rapid, large-scale screening of intestinal parasites in sheep stool samples.

查看原文本刊更多论文

[用于同时检测山羊体内四种肠道寄生虫的多重 PCR 检测方法的开发和初步应用]。

目的方法：根据十二指肠贾第虫（G. duodenalis）（GenBank登录号：XM_001710026.2）、副隐孢子虫（Cryptosporidium parvum）、生物肠虫（Enterocytozoon bieneusi）和莫尼茨虫（Moniezia）的相应基因的保守序列，设计了四对特异性引物：根据十二指肠孢子虫（GenBank登录号：XM_001710026.2）、副隐孢子虫（GenBank登录号：XM_626998.1）、肠孢子虫（GenBank登录号：KJ719492.1) 和莫尼茨绦虫（GenBank登录号：OM296991.1），并开发和优化了同时检测十二指肠球菌、副猪嗜血杆菌、E. bieneusi 和莫尼茨绦虫的多重 PCR 检测方法。在2022年10月至12月期间，从广东省湛江市的4个山羊养殖场共采集了116份新鲜山羊粪便样本，其中96份样本用于评估多重PCR检测方法的检测效果，20份样本作为基线对照进行样本检测。用单靶标PCR检测法和所开发的多重PCR检测法检测96份山羊粪便样本中提取的基因组DNA，并以单靶标PCR检测法为金标准，评估了多重PCR检测法检测山羊粪便样本中十二指肠球菌、副粘病毒、双球菌和莫尼茨绦虫DNA的灵敏度、特异性、阳性预测值和阴性预测值：结果：本研究开发的多重 PCR 检测法可同时扩增十二指肠球菌、副嗜血杆菌、嗜血杆菌和莫尼茨绦虫的特定基因片段。而多重 PCR 法对日本血吸虫、肝片吸虫、粒状棘球蚴、人型布氏囊虫和巴氏杆菌的基因扩增呈阴性。采用单目标 PCR 检测法和所开发的多重 PCR 检测法检测了从 96 份山羊粪便样本中提取的 DNA 样本，单目标 PCR 检测法检测了 40 份山羊粪便样本（41.67%）呈阳性，其中用多重 PCR 检测法检测了 39 份阳性样本，平均吻合率为 97.50%（39/40）。多重 PCR 检测法检测到 26 份山羊粪便样本（27.10%）中的十二指肠球虫 DNA 呈阳性，22 份样本（22.90%）中的副猪嗜血杆菌 DNA 呈阳性，24 份样本（25.00%）中的生物大肠杆菌 DNA 呈阳性，9 份样本（9.40%）中的莫尼茨虫 DNA 呈阳性，这与单靶标 PCR 检测法的检测结果一致。多重 PCR 检测法的灵敏度、阴性预测值和阳性预测值分别为 96.15%、95.83%、100.00% 和 100.00%、98.90%、98.92%、100.00% 和 100.00%、100.00%、100.00%、100.如果将单靶点 PCR 检测作为金标准，则山羊粪便样本中的 G. duodenalis、C. parvum、E. bieneusi 和 Moniezia DNA 的检测灵敏度分别为 98.90%、98.92%、100.00%、100.00% 和 100.00%：结论：已开发出一种高灵敏度和特异性的多重 PCR 检测方法，可同时检测山羊粪便中的 G. duodenalis、C. parvum、E. bieneusi 和 Moniezia，适用于快速、大规模筛查绵羊粪便样本中的肠道寄生虫。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

求助全文

约1分钟内获得全文求助全文

来源期刊

中国血吸虫病防治杂志 Medicine-Medicine (all)

CiteScore

1.30

自引率

0.00%

发文量

7021

期刊介绍： Chinese Journal of Schistosomiasis Control (ISSN: 1005-6661, CN: 32-1374/R), founded in 1989, is a technical and scientific journal under the supervision of Jiangsu Provincial Health Commission and organised by Jiangsu Institute of Schistosomiasis Control. It is a scientific and technical journal under the supervision of Jiangsu Provincial Health Commission and sponsored by Jiangsu Institute of Schistosomiasis Prevention and Control. The journal carries out the policy of prevention-oriented, control-oriented, nationwide and grassroots, adheres to the tenet of scientific research service for the prevention and treatment of schistosomiasis and other parasitic diseases, and mainly publishes academic papers reflecting the latest achievements and dynamics of prevention and treatment of schistosomiasis and other parasitic diseases, scientific research and management, etc. The main columns are Guest Contributions, Experts‘ Commentary, Experts’ Perspectives, Experts' Forums, Theses, Prevention and Treatment Research, Experimental Research, The main columns include Guest Contributions, Expert Commentaries, Expert Perspectives, Expert Forums, Treatises, Prevention and Control Studies, Experimental Studies, Clinical Studies, Prevention and Control Experiences, Prevention and Control Management, Reviews, Case Reports, and Information, etc. The journal is a useful reference material for the professional and technical personnel of schistosomiasis and parasitic disease prevention and control research, management workers, and teachers and students of medical schools. 　　 The journal is now included in important domestic databases, such as Chinese Core List (8th edition), China Science Citation Database (Core Edition), China Science and Technology Core Journals (Statistical Source Journals), and is also included in MEDLINE/PubMed, Scopus, EBSCO, Chemical Abstract, Embase, Zoological Record, JSTChina, Ulrichsweb, Western Pacific Region Index Medicus, CABI and other international authoritative databases.