Rapid and supersensitive allele detection of Plasmodium falciparum chloroquine resistance via a Pyrococcus furiosus argonaute-triggered dual-signal biosensing platform

桑格测序 生物 火球菌属 质粒 恶性疟原虫 聚合酶链反应 抗药性 分子生物学 疟疾 计算生物学 遗传学 病毒学 DNA测序 基因 免疫学 古细菌
作者
Liying Chen,Wencheng Chen,Huagui Wei,Wen‐chang Lin,Cheng Zhang,Haibei Hu,Chunfang Wang,Jiang‐Tao Chen,Xue‐Yan Liang,Daiqian Zhu,Junli Wang,Zongyun Lin,Yuxia Wei,Jian Li,Min Lin
出处
期刊:Parasites & Vectors [BioMed Central]
卷期号:17 (1)
标识
DOI:10.1186/s13071-024-06575-0
摘要

Abstract Background Malaria remains a serious public health problem worldwide, particularly in Africa. Resistance to antimalarial drugs is an essential issue for malaria control and elimination. Currently, polymerase chain reaction (PCR) combined with Sanger sequencing is regarded as the gold standard for mutation detection. However, this method fails to meet the requirements of point-of-care testing (POCT) because of its time-consuming, expensive instruments and professional dependence. To support this strategy, we developed a novel diagnostic platform that combines recombinase polymerase amplification (RPA) with the Pyrococcus furiosus argonaute ( Pf Ago) protein and was designed to detect gene mutations related to antimalarial drug resistance. The Pfcrt haplotypes CVMNK and CVIET of chloroquine resistance (CQR) were used as examples and were assessed in this study. Methods By meticulously designing strategies, RPA primers, guide DNAs, and probes were screened, the reaction was optimized, and the resulting parameters were employed to ascertain the genotype of Pfcrt . The recombinant plasmids pUC57/Pfcrt -CVIET and pUC57/Pfcrt -CVMNK were constructed and diluted for sensitivity detection. The pUC57/Pfcrt -CVIET plasmid mixture was added to the pUC57/Pfcrt -CVMNK plasmid mixture in different additions to configure several specific proportions of mixed plasmid mixtures. The RPA- Pf Ago platform was used, and the mixed plasmid was detected simultaneously via nest-PCR (nPCR) and Sanger sequencing. The platform was then evaluated on 85 clinical samples and compared with Sanger sequencing. Results The entire process achieves the key mutation Pfcrt -CVMNK/CVIET genotype identification of CQR within 90 min. The platform achieved 1.8 × 10 4 copies/μL sensitivity and could detect as little as 3% CVIET in mixed plasmids, which is a higher sensitivity than that of Sanger sequencing (5%). Notably, the platform shows 100% concordance with the gold standard method when 85 clinical samples are tested. The sensitivity and specificity were 100% for the 85 clinical samples. Conclusions This study established an RPA- Pf Ago platform for genotyping the key mutation Pfcrt -CVMNK/CVIET of CQR. This method can rapidly produce reliable results and avoid the disadvantages of nPCR with sequencing. This approach has the characteristics of a short operation time, low device dependence, and a good match to the POCT strategy, suggesting that the platform can be easily applied locally or on site. Graphical abstract

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