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冈比亚按蚊中杀虫剂抗性突变的检测与监测:个体样本与混合样本对比

Detection and Monitoring of Insecticide Resistance Mutations in Anopheles gambiae: Individual vs Pooled Specimens.

作者信息

Mavridis Konstantinos, Wipf Nadja, Müller Pie, Traoré Mohamed M, Muller Gunter, Vontas John

机构信息

Institute of Molecular Biology and Biotechnology, Foundation for Research and Technology-Hellas, 70013 Heraklion, Greece.

Department of Epidemiology and Public Health, Swiss Tropical and Public Health Institute, Socinstrasse 57, 4002 Basel, Switzerland.

出版信息

Genes (Basel). 2018 Oct 3;9(10):479. doi: 10.3390/genes9100479.

DOI:10.3390/genes9100479
PMID:30282959
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6209882/
Abstract

Bioassays and molecular diagnostics are routinely used for the monitoring of malaria vector populations to support insecticide resistance management (IRM), guiding operational decisions on which insecticides ought to be used for effective vector control. Previously developed TaqMan assays were optimised to distinguish the wild-type L1014 from the knockdown resistance () point mutations 1014F and 1014S (triplex reaction), and the N1575 wild-type from the point mutation 1575Y (duplex reaction). Subsequently, artificial pools of specimens with known genotypes of L1014F, L1014S, and N1575Y were created, nucleic acids were extracted, and mutations were detected. These data were then used to define a linear regression model that predicts the allelic frequency within a pool of mosquitoes as a function of the measured ΔCt values (Ct mutant - Ct wild type probe). Polynomial regression models showed values of >0.99 ( < 0.05). The method was validated with populations of variable allelic frequencies, and found to be precise (1.66⁻2.99%), accurate (3.3⁻5.9%), and able to detect a single heterozygous mosquito mixed with 9 wild type individuals in a pool of 10. Its pilot application in field-caught samples showed minimal differences from individual genotyping (0.36⁻4.0%). It allowed the first detection of the super- mutation N1575Y in from Mali. Using pools instead of individuals allows for more efficient resistance allele screening, facilitating IRM.

摘要

生物测定和分子诊断常用于监测疟疾媒介种群,以支持杀虫剂抗性管理(IRM),为有效控制媒介应使用何种杀虫剂的操作决策提供指导。先前开发的TaqMan测定法经过优化,可区分野生型L1014与击倒抗性()点突变1014F和1014S(三重反应),以及N1575野生型与点突变1575Y(双重反应)。随后,创建了具有已知L1014F、L1014S和N1575Y基因型的人工样本池,提取核酸,并检测突变。然后使用这些数据定义一个线性回归模型,该模型根据测量的ΔCt值(Ct突变体 - Ct野生型探针)预测蚊子样本池中等位基因频率。多项式回归模型显示R值>0.99(P<0.05)。该方法在等位基因频率不同的种群中得到验证,发现其精确(1.66⁻2.99%)、准确(3.3⁻5.9%),并且能够在10只蚊子的样本池中检测到与9只野生型个体混合的单只杂合蚊子。其在野外捕获样本中的初步应用显示与个体基因分型的差异极小(0.36⁻4.0%)。它首次在来自马里的样本中检测到超级突变N1575Y。使用样本池而非个体进行检测可实现更高效的抗性等位基因筛查,便于进行杀虫剂抗性管理。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2bba/6209882/0c22631401b3/genes-09-00479-g001a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2bba/6209882/0c22631401b3/genes-09-00479-g001a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2bba/6209882/0c22631401b3/genes-09-00479-g001a.jpg

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