Temeyer Kevin B, Tong Fan, Totrov Maxim M, Tuckow Alexander P, Chen Qiao-hong, Carlier Paul R, Pérez de León Adalberto A, Bloomquist Jeffrey R
Agricultural Research Service, U. S. Department of Agriculture, Knipling-Bushland U.S. Livestock Insects Research Laboratory, 2700 Fredericksburg Road, Kerrville, TX, 78028-9184, USA.
Department of Entomology and Nematology, Emerging Pathogens Institute, University of Florida, 2055 Mowry Road, PO Box 100009, Gainesville, FL, 32610-00009, USA.
Parasit Vectors. 2014 Dec 10;7:577. doi: 10.1186/s13071-014-0577-4.
Phlebotomus papatasi vectors zoonotic cutaneous leishmaniasis. Previous expression of recombinant P. papatasi acetylcholinesterase (PpAChE1) revealed 85% amino acid sequence identity to mosquito AChE and identified synthetic carbamates that effectively inhibited PpAChE1 with improved specificity for arthropod AChEs compared to mammalian AChEs. We hypothesized that the G119S mutation causing high level resistance to organophosphate insecticides in mosquitoes may occur in PpAChE1 and may reduce sensitivity to inhibition. We report construction, expression, and biochemical properties of rPpAChE1 containing the G119S orthologous mutation.
Targeted mutagenesis introduced the G119S orthologous substitution in PpAChE1 cDNA. Recombinant PpAChE1 enzymes containing or lacking the G119S mutation were expressed in the baculoviral system. Biochemical assays were conducted to determine altered catalytic properties and inhibitor sensitivity resulting from the G119S substitution. A molecular homology model was constructed to examine the modeled structural interference with docking of inhibitors of different classes. Genetic tests were conducted to determine if the G119S orthologous codon existed in polymorphic form in a laboratory colony of P. papatasi.
Recombinant PpAChE1 containing the G119S substitution exhibited altered biochemical properties, and reduced inhibition by compounds that bind to the acylation site on the enzyme (with the exception of eserine). Less resistance was directed against bivalent or peripheral site inhibitors, in good agreement with modeled inhibitor docking. Eserine appeared to be a special case capable of inhibition in the absence of covalent binding at the acylation site. Genetic tests did not detect the G119S mutation in a laboratory colony of P. papatasi but did reveal that the G119S codon existed in polymorphic form (GGA + GGC).
The finding of G119S codon polymorphism in a laboratory colony of P. papatasi suggests that a single nucleotide transversion (GGC → AGC) may readily occur, causing rapid development of resistance to organophosphate and phenyl-substituted carbamate insecticides under strong selection. Careful management of pesticide use in IPM programs is important to prevent or mitigate development and fixation of the G119S mutation in susceptible pest populations. Availability of recombinant AChEs enables identification of novel inhibitory ligands with improved efficacy and specificity for AChEs of arthropod pests.
巴氏白蛉是动物源性皮肤利什曼病的传播媒介。此前对重组巴氏白蛉乙酰胆碱酯酶(PpAChE1)的表达研究显示,其与蚊虫乙酰胆碱酯酶有85%的氨基酸序列同一性,并鉴定出了一些合成氨基甲酸酯类化合物,这些化合物能有效抑制PpAChE1,与哺乳动物乙酰胆碱酯酶相比,对节肢动物乙酰胆碱酯酶具有更高的特异性。我们推测,导致蚊虫对有机磷杀虫剂产生高水平抗性的G119S突变可能发生在PpAChE1中,并可能降低其对抑制作用的敏感性。我们报告了含有G119S同源突变的重组PpAChE1的构建、表达及生化特性。
通过定点诱变在PpAChE1 cDNA中引入G119S同源替换。含有或缺乏G119S突变的重组PpAChE1酶在杆状病毒系统中表达。进行生化分析以确定G119S替换导致的催化特性和抑制剂敏感性的改变。构建分子同源模型以研究对不同类抑制剂对接的模拟结构干扰。进行基因检测以确定G119S同源密码子在巴氏白蛉实验室种群中是否以多态形式存在。
含有G119S替换的重组PpAChE1表现出改变的生化特性,对与酶酰化位点结合的化合物的抑制作用降低(除了毒扁豆碱)。对二价或外周位点抑制剂的抗性较小,这与模拟的抑制剂对接结果高度一致。毒扁豆碱似乎是一个特殊情况,在酰化位点不存在共价结合的情况下仍能产生抑制作用。基因检测在巴氏白蛉实验室种群中未检测到G119S突变,但确实发现G119S密码子以多态形式存在(GGA + GGC)。
在巴氏白蛉实验室种群中发现G119S密码子多态性表明,单个核苷酸颠换(GGC → AGC)可能很容易发生,在强烈选择下会导致对有机磷和苯基取代氨基甲酸酯类杀虫剂的抗性快速发展。在综合虫害管理计划中谨慎管理农药使用对于防止或减轻易感害虫种群中G119S突变的发展和固定很重要。重组乙酰胆碱酯酶的可用性使得能够鉴定出对节肢动物害虫乙酰胆碱酯酶具有更高效力和特异性的新型抑制性配体。
Zotero 插件
