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A single mutation in the GSTe2 gene allows tracking of metabolically-based insecticide resistance in a major malaria vector

机译:GSTe2基因中的单个突变允许追踪主要疟疾载体中基于代谢的杀虫剂抗性

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摘要

Background\ud\udMetabolic resistance to insecticides is the biggest threat to the continued effectiveness of malaria vector control. However, its underlying molecular basis, crucial for successful resistance management, remains poorly characterized.\ud\udResults\ud\udHere, we demonstrate that the single amino acid change L119F in an upregulated glutathione S-transferase gene, GSTe2, confers high levels of metabolic resistance to DDT in the malaria vector Anopheles funestus. Genome-wide transcription analysis revealed that GSTe2 was the most over-expressed detoxification gene in DDT and permethrin-resistant mosquitoes from Benin. Transgenic expression of GSTe2 in Drosophila melanogaster demonstrated that over-transcription of this gene alone confers DDT resistance and cross-resistance to pyrethroids. Analysis of GSTe2 polymorphism established that the point mutation is tightly associated with metabolic resistance to DDT and its geographical distribution strongly correlates with DDT resistance patterns across Africa. Functional characterization of recombinant GSTe2 further supports the role of the L119F mutation, with the resistant allele being more efficient at metabolizing DDT than the susceptible one. Importantly, we also show that GSTe2 directly metabolizes the pyrethroid permethrin. Structural analysis reveals that the mutation confers resistance by enlarging the GSTe2 DDT-binding cavity, leading to increased DDT access and metabolism. Furthermore, we show that GSTe2 is under strong directional selection in resistant populations, and a restriction of gene flow is observed between African regions, enabling the prediction of the future spread of this resistance.\ud\udConclusions\ud\udThis first DNA-based metabolic resistance marker in mosquitoes provides an essential tool to track the evolution of resistance and to design suitable resistance management strategies.
机译:背景\对杀虫剂的新陈代谢抗性是对疟疾媒介控制的持续有效性的最大威胁。但是,其对于成功进行抗药性管理至关重要的潜在分子基础仍然缺乏良好的表征。\ ud \ udResults \ ud \ ud在这里,我们证明了谷胱甘肽S-转移酶基因GSTe2中单个氨基酸的L119F改变赋予了高水平的谷胱甘肽S-转移酶基因疟疾媒介按蚊中对滴滴涕的代谢抗性。全基因组转录分析表明,GSTe2是贝宁的DDT和耐氯菊酯的蚊子中最过量表达的解毒基因。果蝇中GSTe2的转基因表达表明,仅该基因的过度转录赋予DDT抗药性和对拟除虫菊酯的交叉抗性。对GSTe2多态性的分析确定,点突变与对DDT的代谢抗性紧密相关,并且其地理分布与整个非洲的DDT抗性模式密切相关。重组GSTe2的功能表征进一步支持L119F突变的作用,抗性等位基因在DDT代谢方面比易感等位基因更有效。重要的是,我们还显示了GSTe2直接代谢拟除虫菊酯苄氯菊酯。结构分析表明,该突变通过扩大GSTe2 DDT结合腔而赋予抗性,从而导致DDT的获得和代谢增加。此外,我们表明,GSTe2在抗性种群中处于强方向选择,并且在非洲区域之间观察到基因流的限制,从而能够预测这种抗性的未来传播。\ ud \ ud结论\ ud \ ud这第一个基于DNA的蚊子中的代谢抗性标记物提供了跟踪抗性演变和设计合适的抗性管理策略的重要工具。

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