Restriction fragment length polymorphism analysis of genes of virulent strain isolate of Toxoplasma gondii using enzyme DdeI

Q2 Veterinary

International Journal of One Health Pub Date : 2021-01-01 DOI:10.14202/ijoh.2021.196-203

F. Ekawasti, U. Cahyaningsih, N. Dharmayanti, S. Sa’diah, D. Subekti, Z. Azmi, M. I. Desem

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引用次数: 1

Abstract

Background and Aim: Toxoplasma gondii is a unicellular coccidian parasite distributed globally and is an important zoonotic pathogen. Approximately 30% of the human population worldwide is chronically infected with T. gondii. The pathogenicity of this species depends on the type originating from the clonal population. Techniques for more accurately determining the type of T. gondii have recently been developed using genetic markers. Specifically, T. gondii has been typed using polymerase chain reaction-restriction fragment length polymorphism (PCR-RFLP). This study aimed to identify sets of PCR-RFLP markers that have high power to discriminate genotyping of T. gondii and are easy to use and are easy to use. The objective of this study was to characterize virulent strain isolates of T. gondii by PCR-RFLP using 10 markers with DdeI. Materials and Methods: T. gondii tachyzoites (RH virulent strain) were derived from culture cells at the Indonesian Research Center for Veterinary Sciences. Genotyping was performed on T. gondii DNA extracted from cell cultured tachyzoites using 10 genetic markers of PCR-RFLP, namely, B1#1, B1#2, B1#3, SAG1#1, SAG1#2, P30, BAG1, ROP1, GRA1, and GRA7, with digestion using the restriction enzyme DdeI. Results: The 10 genes were amplified by PCR. Among them, three genetic markers, B1#3, ROP1, and GRA1, were genotyped by the PCR-RFLP using restriction enzyme DdeI. Overall, the findings showed that the specific RFLP profile of digestion of gene regions by DdeI could be used as a specific marker for the virulent biotype causative of toxoplasmosis. In addition, virulent strains of T. gondii can be easily detected by these markers. Conclusion: Three pairs of primers (B1#3, ROP1, and GRA1) with DdeI have proven useful for the diagnosis of acute toxoplasmosis (virulent strain biotype I). This proposed method is relatively simple, rapid, cheap, and can be performed in most laboratories, providing a practical approach for the routine analysis of T. gondii strains.

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用DdeI酶分析刚地弓形虫毒力分离株基因的限制性内切片段长度多态性

背景与目的:刚地弓形虫是一种分布于全球的单细胞球虫寄生虫，是一种重要的人畜共患病原体。全世界大约30%的人口慢性感染了弓形虫。该物种的致病性取决于源自克隆种群的类型。最近已经开发出利用遗传标记更准确地确定弓形虫类型的技术。具体来说，弓形虫已经使用聚合酶链反应-限制性片段长度多态性(PCR-RFLP)进行了分型。本研究旨在寻找一组对弓形虫基因分型判别能力强、操作简单、使用方便的PCR-RFLP标记。本研究的目的是采用PCR-RFLP方法，利用10个带有DdeI的标记物对弓形虫毒力菌株进行鉴定。材料与方法:刚地弓形虫速殖子(RH毒株)来源于印度尼西亚兽医科学研究中心的培养细胞。利用PCR-RFLP的10个遗传标记，分别为B1#1、B1#2、B1#3、SAG1#1、SAG1#2、P30、BAG1、ROP1、GRA1和GRA7，对从细胞培养的速殖子中提取的弓形虫DNA进行基因分型，并使用DdeI酶切。结果:PCR扩增出10个基因。其中B1#3、ROP1和GRA1 3个遗传标记采用限制性内切酶DdeI进行PCR-RFLP分型。综上所述，DdeI酶切基因区域的特异性RFLP谱可作为弓形虫病毒力型病原体的特异性标记物。此外，这些标记可以很容易地检测出弓形虫的毒力菌株。结论:3对DdeI引物(B1#3、ROP1和GRA1)可用于诊断急性弓形虫病(I型毒株)，该方法简便、快速、廉价，可在大多数实验室进行，为弓形虫的常规分析提供了一种实用的方法。

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来源期刊

International Journal of One Health Veterinary-Veterinary (all)

CiteScore

2.10

自引率

0.00%

发文量

审稿时长

15 weeks

期刊介绍： International Journal of One Health publishes high quality and novelty papers focusing on One Health. Review articles are highly appreciated. All articles published by International Journal of One Health are made freely and permanently accessible online. All articles to International Journal of One Health are posted online immediately as they are ready for publication.