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首页> 外文OA文献 >Resistance of Trichoplusia ni to Bacillus thuringiensis Toxin Cry1Ac Is Independent of Alteration of the Cadherin-Like Receptor for Cry Toxins
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Resistance of Trichoplusia ni to Bacillus thuringiensis Toxin Cry1Ac Is Independent of Alteration of the Cadherin-Like Receptor for Cry Toxins

机译:毛滴虫对苏云金芽孢杆菌毒素Cry1Ac的抗性独立于Cadherin受体对Cry毒素的改变

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Alteration of binding sites for Bacillus thuringiensis (Bt) toxins in insect midgut is the major mechanism of high-level resistance to Bt toxins in insects. The midgut cadherin is known to be a major binding protein for Bt Cry1A toxins and linkage of Bt-resistance to cadherin gene mutations has been identified in lepidopterans. The resistance to Bt toxin Cry1Ac evolved in greenhouse populations of Trichoplusia ni has been identified to be associated with the down-regulation of an aminopeptidase N (APN1) gene by a trans-regulatory mechanism and the resistance gene has been mapped to the locus of an ABC transporter (ABCC2) gene. However, whether cadherin is also involved with Cry1Ac-resistance in T. ni requires to be understood. Here we report that the Cry1Ac-resistance in T. ni is independent of alteration of the cadherin. The T. ni cadherin cDNA was cloned and the cadherin sequence showed characteristic features known to cadherins from Lepidoptera. Various T. ni cadherin gene alleles were identified and genetic linkage analysis of the cadherin alleles with Cry1Ac-resistance showed no association of the cadherin gene with the Cry1Ac-resistance in T. ni. Analysis of cadherin transcripts showed no quantitative difference between the susceptible and Cry1Ac-resistant T. ni larvae. Quantitative proteomic analysis of midgut BBMV proteins by iTRAQ-2D-LC-MS/MS determined that there was no quantitative difference in cadherin content between the susceptible and the resistant larvae and the cadherin only accounted for 0.0014% (mol%) of the midgut BBMV proteins, which is 1/300 of APN1 in molar ratio. The cadherin from both the susceptible and resistant larvae showed as a 200-kDa Cry1Ac-binding protein by toxin overlay binding analysis, and nano-LC-MS/MS analysis of the 200-kDa cadherin determined that there is no quantitative difference between the susceptible and resistant larvae. Results from this study indicate that the Cry1Ac-resistance in T. ni is independent of cadherin alteration.
机译:昆虫中肠中苏云金芽孢杆菌(Bt)毒素结合位点的改变是昆虫对Bt毒素产生高水平抗性的主要机制。已知中肠钙粘着蛋白是Bt Cry1A毒素的主要结合蛋白,在鳞翅目中已确定Bt抗性与钙粘着蛋白基因突变的联系。已经确定,对温室滴虫Trichoplusia ni的Bt毒素Cry1Ac的抗性通过反调节机制与氨基肽酶N(APN1)基因的下调相关,并且该抗性基因已被定位到一个特定的地方。 ABC转运蛋白(ABCC2)基因。但是,钙粘着蛋白是否也与T. ni中的Cry1Ac抗性有关。在这里,我们报告在T. ni中的Cry1Ac抗性与钙粘蛋白的变化无关。克隆了T. ni钙粘蛋白cDNA,并且钙粘蛋白序列显示了鳞翅目钙粘蛋白已知的特征。鉴定了多种T. ni钙粘蛋白基因等位基因,并且对具有Cry1Ac抗性的钙粘蛋白等位基因进行了遗传连锁分析,结果表明,钙粘蛋白基因与C.1Ac抗性没有关联。钙粘蛋白转录本的分析显示,易感和耐Cry1Ac的T. ni幼虫之间没有定量差异。通过iTRAQ-2D-LC-MS / MS对中肠BBMV蛋白质组蛋白进行定量分析,确定易感幼虫和抗性幼虫之间的钙粘着蛋白含量没有定量差异,而钙粘着蛋白仅占中肠BBMV的0.0014%(mol%)蛋白质,摩尔比为APN1的1/300。易感幼虫和抗性幼虫中的钙黏着蛋白通过毒素覆盖结合分析显示为200 kDa Cry1Ac结合蛋白,并且200 kDa钙黏着蛋白的纳米LC-MS / MS分析确定易感性之间没有定量差异和抗性幼虫。这项研究的结果表明,T。ni中的Cry1Ac抗性与钙粘蛋白改变无关。

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