Molecular analysis of resistance to acaricidal spirocyclic tetronic acids in Tetranychus urticae: CYP392E10 metabolizes spirodiclofen, but not its corresponding enol

被引:118
作者
Demaeght, Peter [1 ]
Dermauw, Wannes [1 ]
Tsakireli, Dimitra [2 ]
Khajehali, Jahangir [1 ]
Nauen, Ralf [3 ,4 ]
Tirry, Luc [1 ]
Vontas, John [2 ]
Luemmen, Peter [4 ,5 ]
Van Leeuwen, Thomas [1 ]
机构
[1] Univ Ghent, Fac Biosci Engn, Dept Crop Protect, B-9000 Ghent, Belgium
[2] Univ Crete, Dept Biol, Fac Appl Biol & Biotechnol, Iraklion 71409, Greece
[3] BayerCropSci AG, Res Pest Control, D-40789 Monheim, Germany
[4] Germany Bayer CropSci, Monheim, Germany
[5] BayerCropSci AG, Biochem, D-40789 Monheim, Germany
关键词
Mode of action; Induction; Detoxification; Cooperative binding; Adaptation; Selection; 2-SPOTTED SPIDER-MITE; ACETYL-COA CARBOXYLASE; ANOPHELES-GAMBIAE; HETEROTROPIC COOPERATIVITY; INSECTICIDE RESISTANCE; FIELD POPULATIONS; CROSS-RESISTANCE; BEMISIA-TABACI; SPIROMESIFEN; SUSCEPTIBILITY;
D O I
10.1016/j.ibmb.2013.03.007
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Spirodiclofen is one of the most recently developed acaricides and belongs to the new family of spirocyclic tetronic acids (ketoenols). This new acaricidal family is an important chemical tool in resistance management strategies providing sustainable control of spider mites such as Tetranychus urticae. Spirodiclofen targets lipid biosynthesis mediated by direct inhibition of acetyl coenzyme A carboxylase (ACCase). In this study, we investigated two genetically distant spider mite strains with high resistance to spirodiclofen. Despite the strong resistance levels to spirodiclofen (up to 680-fold), only limited cross-resistance with other members of this group such as spiromesifen and spirotetramat could be detected. Amplification and sequencing of the ACCase gene from resistant and susceptible strains did not reveal common non-synonymous mutations, and expression levels of ACCase were similar in both resistant and susceptible strains, indicating the absence of target-site resistance. Furthermore, we collected genome-wide expression data of susceptible and resistant T. urticae strains using microarray technology. Analysis of differentially expressed genes revealed a broad response, but within the overlap of two resistant strains, several cytochrome P450s were prominent. Quantitative PCR confirmed the constitutive over-expression of CYP392E7 and CYP392E10 in resistant strains, and CYP392E10 expression was highly induced by spirodiclofen. Furthermore, stage specific expression profiling revealed that expression levels were not significantly different between developing stages, but very low in eggs, matching the age-dependent resistance pattern previously observed. Functional expression of CYP392E7 and CYP392E10 confirmed that CYP392E10 (but not CYP392E7) metabolizes spirodidofen by hydroxylation as identified by LC-MS/MS, and revealed cooperative substrate binding and a K-m of 43 mu M spirodiclofen. CYP392E10 also metabolizes spiromesifen, but not spirotetramat. Surprisingly, no metabolism of the hydrolyzed spirodiclofen-enol metabolite could be detected. These findings are discussed in the light of a likely resistance mechanism. (C) 2013 Elsevier Ltd. All rights reserved.
引用
收藏
页码:544 / 554
页数:11
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