首页> 美国卫生研究院文献>Toxins >The Cadherin Cry1Ac Binding-Region is Necessary for the Cooperative Effect with ABCC2 Transporter Enhancing Insecticidal Activity of Bacillus thuringiensis Cry1Ac Toxin
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The Cadherin Cry1Ac Binding-Region is Necessary for the Cooperative Effect with ABCC2 Transporter Enhancing Insecticidal Activity of Bacillus thuringiensis Cry1Ac Toxin

机译:Cadherin Cry1Ac结合区域是与ABCC2转运蛋白增强苏云金芽孢杆菌Cry1Ac毒素杀虫活性的协同作用所必需的

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摘要

Bacillus thuringiensis Cry1Ac toxin binds to midgut proteins, as cadherin (CAD) and ABCC2 transporter, to form pores leading to larval death. In cell lines, co-expression of CAD and ABCC2 enhance Cry1Ac toxicity significantly, but the mechanism remains elusive. Here, we show that the expression of Helicoverpa armigera CAD (HaCAD-GFP) in Hi5 cells induces susceptibility to Cry1Ac and enhanced Cry1Ac toxicity when co-expressed with H. armigera ABCC2 (HaABCC2-GFP), since Cry1Ac toxicity increased 735-fold compared to Hi5 cells expressing HaCAD-GFP alone or 28-fold compared to HaABCC2-GFP alone. In contrast, the expression of the Spodoptera litura CAD (SlCAD-GFP) in Hi5 cells did not induce susceptibility to Cry1Ac nor it potentiated Cry1Ac toxicity with HaABCC2-GFP. To identify the CAD regions involved in the enhancement of Cry1Ac toxicity with ABCC2, the different CAD domains were replaced between SlCAD-GFP and HaCad-GFP proteins, and cytotoxicity assays were performed in Hi5 cells in the absence or presence of HaABCC2-GFP. The HaCAD toxin-binding region (TB), specifically the CAD repeat-11, was necessary to enhance Cry1Ac toxicity with ABCC2. We propose that CAD TB is involved in recruiting Cry1Ac to localize it in a good position for its interaction with the ABCC2, resulting in efficient toxin membrane insertion enhancing Cry1Ac toxicity.
机译:苏云金芽孢杆菌的Cry1Ac毒素与中肠蛋白(如钙黏着蛋白(CAD)和ABCC2转运蛋白)结合,形成导致幼虫死亡的孔。在细胞系中,CAD和ABCC2的共表达可显着增强Cry1Ac的毒性,但机制尚不清楚。在这里,我们显示棉铃虫CAD(HaCAD-GFP)在Hi5细胞中的表达诱导与棉铃虫ABCC2(HaABCC2-GFP)共表达时对Cry1Ac的敏感性和增强的Cry1Ac毒性,因为与之相比,Cry1Ac毒性增加了735倍单独表达HaCAD-GFP或比单独HaABCC2-GFP的表达高28倍的H5细胞。相反,斜纹夜蛾CAD(SlCAD-GFP)在Hi5细胞中的表达不会诱导对Cry1Ac的敏感性,也不会增强HaABCC2-GFP对Cry1Ac的毒性。为了鉴定涉及用ABCC2增强Cry1Ac毒性的CAD区域,在SlCAD-GFP和HaCad-GFP蛋白之间替换了不同的CAD结构域,并在不存在或存在HaABCC2-GFP的情况下在Hi5细胞中进行了细胞毒性测定。 HaCAD毒素结合区(TB),特别是CAD repeat-11,对于增强Cry1Ac对ABCC2的毒性是必需的。我们建议CAD TB参与募集Cry1Ac,使其定位在与ABCC2相互作用的良好位置,从而有效地插入毒素膜,从而增强Cry1Ac的毒性。

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