Rapid detection of mutations in the suspected piperaquine resistance gene E415G-exo in Plasmodium falciparum exonuclease via AS‒PCR and RAA with CRISPR/Cas12a

IF 4.1 2区 医学 Q1 PARASITOLOGY
Huiyin Zhu , Daiqian Zhu , Yuting Li , Yun Li , Xiaonan Song , Jinyu Mo , Long Liu , Zhixin Liu , Siqi Wang , Yi Yao , He Yan , Kai Wu , Wei Wang , Jianhai Yin , Min Lin , Jian Li
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Abstract

Malaria remains a major public health concern. The rapid spread of resistance to antimalarial drugs is a major challenge for malaria eradication. Timely and accurate molecular monitoring based on practical detection methods is a critical step toward malaria control and elimination. In this study, two rapid detection techniques, allele-specific PCR (ASPCR) and recombinase-aided amplification (RAA) combined with CRISPR/Cas12a, were established, optimized and assessed to detect single nucleotide polymorphisms in the Plasmodium falciparum exonuclease (Pfexo) gene related to suspected piperaquine resistance. Moreover, phosphorothioate and artificial mismatches were introduced into the allele-specific primers for ASPCR, and crRNA-mismatched bases were introduced into the RAACRISPR/Cas12a assay because crRNAs designed according to conventional rules fail to discriminate genotypes. As a result, the detection limits of the ASPCR and RAACRISPR/Cas12a assays were 104 copies/μL and 103 copies/μL, respectively. The detection threshold for dried blood spots was 100150 parasites/μL, with no cross-reactivity against other genotypes. The average cost of ASPCR is approximately $1 per test and takes 23 h, whereas that of the RAACRISPR/Cas12a system is approximately $7 per test and takes 1 h or less. Therefore, we provide more options for testing single nucleotide polymorphisms in the Pfexo gene, considering economic conditions and the availability of instruments, equipment, and reagents, which can contribute to the molecular monitoring of antimalarial resistance.

Abstract Image

通过 AS-PCR 和 CRISPR/Cas12a RAA 快速检测恶性疟原虫外切酶中疑似哌喹抗性基因 E415G-exo 的突变。
疟疾仍然是一个重大的公共卫生问题。抗疟药物抗药性的迅速蔓延是根除疟疾的一大挑战。基于实用检测方法的及时准确的分子监测是控制和消除疟疾的关键一步。本研究建立、优化并评估了两种快速检测技术,即等位基因特异性 PCR(AS-PCR)和结合 CRISPR/Cas12a 的重组酶辅助扩增(RAA),用于检测恶性疟原虫外切酶(Pfexo)基因中与疑似哌喹抗药性相关的单核苷酸多态性。此外,在 AS-PCR 的等位基因特异引物中引入了硫代磷酸酯和人工错配,在 RAA-CRISPR/Cas12a 检测中引入了 crRNA 错配碱基,因为按照传统规则设计的 crRNA 无法区分基因型。因此,AS-PCR 和 RAA-CRISPR/Cas12a 检测方法的检测限分别为 104 个拷贝/μL 和 103 个拷贝/μL。干血斑的检测阈值为 100-150 个寄生虫/μL,对其他基因型无交叉反应。AS-PCR每次检测的平均成本约为1美元,耗时2-3小时,而RAA-CRISPR/Cas12a系统每次检测的平均成本约为7美元,耗时1小时或更短。因此,考虑到经济条件以及仪器、设备和试剂的可用性,我们为检测 Pfexo 基因的单核苷酸多态性提供了更多的选择,有助于对抗疟药物耐药性的分子监测。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
CiteScore
7.90
自引率
7.50%
发文量
31
审稿时长
48 days
期刊介绍: The International Journal for Parasitology – Drugs and Drug Resistance is one of a series of specialist, open access journals launched by the International Journal for Parasitology. It publishes the results of original research in the area of anti-parasite drug identification, development and evaluation, and parasite drug resistance. The journal also covers research into natural products as anti-parasitic agents, and bioactive parasite products. Studies can be aimed at unicellular or multicellular parasites of human or veterinary importance.
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