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与拉丁美洲埃及伊蚊拟除虫菊酯抗性相关的电压门控钠通道基因突变。

A mutation in the voltage-gated sodium channel gene associated with pyrethroid resistance in Latin American Aedes aegypti.

作者信息

Saavedra-Rodriguez K, Urdaneta-Marquez L, Rajatileka S, Moulton M, Flores A E, Fernandez-Salas I, Bisset J, Rodriguez M, McCall P J, Donnelly M J, Ranson H, Hemingway J, Black W C

机构信息

Department of Microbiology, Immunology and Pathology, Colorado State University, Fort Collins, CO, USA.

出版信息

Insect Mol Biol. 2007 Dec;16(6):785-98. doi: 10.1111/j.1365-2583.2007.00774.x.

Abstract

Pyrethroids are commonly used as mosquito adulticides and evolution of resistance to these compounds is a major threat to public health. 'Knockdown resistance' to pyrethroids (kdr) is frequently caused by nonsynonymous mutations in the voltage-gated sodium channel transmembrane protein (para) that reduce pyrethroid binding. Early detection of kdr is critical to the development of resistance management strategies in mosquitoes including Aedes aegypti, the most prevalent vector of dengue and yellow fever viruses. Brengues et al. described seven novel mutations in hydrophobic segment 6 of domain II of para in Ae. aegypti. Assays on larvae from strains bearing these mutations indicated reduced nerve sensitivity to permethrin inhibition. Two of these occurred in codons Iso1011 and Val1016 in exons 20 and 21 respectively. A transition in the third position of Iso1011 encoded a Met1011 replacement and a transversion in the second position of Val1016 encoded a Gly1016 replacement. We have screened this same region in 1318 mosquitoes in 32 additional strains; 30 from throughout Latin America. While the Gly1016 allele was never detected in Latin America, we found two new mutations in these same codons. A transition in the first position of codon 1011 encodes a Val replacement while a transition in the first position of codon 1016 encodes an Iso replacement. We developed PCR assays for these four mutations that can be read either on an agarose gel or as a melting curve. Selection experiments, one with deltamethrin on a field strain from Santiago de Cuba and another with permethrin on a strain from Isla Mujeres, Mexico rapidly increased the frequency of the Iso1016 allele. Bioassays of F(3) offspring arising from permethrin susceptible Val1016 homozygous parents and permethrin resistant Iso1016 homozygous parents show that Iso1016 segregates as a recessive allele in conferring kdr. Analysis of segregation between alleles at the 1011 and 1016 codons in the F(3) showed a high rate of recombination even though the two codons are only separated by a ~250 bp intron. The tools and information presented provide a means for early detection and characterization of kdr that is critical to the development of strategies for resistance management.

摘要

拟除虫菊酯通常用作灭蚊成虫剂,对这些化合物产生抗药性的进化是对公共卫生的重大威胁。对拟除虫菊酯的“击倒抗性”(kdr)通常由电压门控钠通道跨膜蛋白(para)中的非同义突变引起,这些突变会减少拟除虫菊酯的结合。早期检测kdr对于制定包括埃及伊蚊(登革热和黄热病病毒最主要的传播媒介)在内的蚊子抗药性管理策略至关重要。布伦格斯等人描述了埃及伊蚊para基因结构域II疏水片段6中的七个新突变。对携带这些突变的品系的幼虫进行的检测表明,其神经对氯菊酯抑制的敏感性降低。其中两个分别发生在外显子20和21的密码子Iso1011和Val1016中。Iso1011第三位的转换编码了Met1011的替换,Val1016第二位的颠换编码了Gly1016的替换。我们在另外32个品系的1318只蚊子中筛选了同一区域;其中30个来自拉丁美洲各地。虽然在拉丁美洲从未检测到Gly1016等位基因,但我们在相同密码子中发现了两个新突变。密码子1011第一位的转换编码了Val的替换,而密码子1016第一位的转换编码了Iso的替换。我们针对这四个突变开发了PCR检测方法,可在琼脂糖凝胶上读取或作为熔解曲线读取。选择实验,一个是对来自古巴圣地亚哥的野外品系使用溴氰菊酯,另一个是对来自墨西哥穆赫雷斯岛的品系使用氯菊酯,迅速增加了Iso1016等位基因的频率。对氯菊酯敏感的Val1016纯合亲本和氯菊酯抗性的Iso1016纯合亲本产生的F(3)后代进行的生物测定表明,Iso1016作为隐性等位基因在赋予kdr方面进行分离。对F(3)中1011和1016密码子处等位基因之间的分离分析表明,即使这两个密码子仅被一个约250 bp的内含子隔开,重组率也很高。所提供的工具和信息为kdr的早期检测和特征描述提供了一种手段,这对于抗药性管理策略的制定至关重要。

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