首页> 外文期刊>The FEBS journal >A second independent resistance mechanism to Bacillus sphaericus binary toxin targets its alpha-glucosidase receptor in Culex quinquefasciatus
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A second independent resistance mechanism to Bacillus sphaericus binary toxin targets its alpha-glucosidase receptor in Culex quinquefasciatus

机译:对球形芽孢杆菌二元毒素的第二种独立抗性机制,以库蚊(Culex quinquefasciatus)中的α-葡萄糖苷酶受体为目标

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摘要

The entomopathogen Bacillus sphaericus is an important tool for the vector control of Culex sp., and its effectiveness has been validated in field trials. The appearance of resistance to this bacterium, however, remains a threat to its use, and attempts have been made to understand the resistance mechanisms. Previous work showed that the resistance to B. sphaericus in a Culex qu inquefascia tits colony is associated with the absence of the approximate to 60-kDa binary toxin receptor in larvae midgut microvilli. Here, the gene encoding the C. quinquefasciatus toxin receptor, Cqm1, was cloned and sequenced from a Susceptible colony. The deduced amino-acid sequence confirmed its identity as an alpha-glucosidase, and analysis of the corresponding gene sequence from resistant larvae implicated a 19-nucleotide deletion as the basis for resistance. This deletion changes the ORF and originates a premature stop codon, which prevents the synthesis of the full-length Cqm1. Expression of the truncated protein, however, was not detected when whole larvae extracts were probed with antibodies raised against an N-terminal 45-kDa recombinant fragment of Cqm1. It seems that the premature stop codon directs the Mutated cqm1 to the nonsense-mediated decay pathway of mRNA degradation. In-gel assays confirmed that a single alpha-glucosidase protein is missing from the resistant colony. Further in vitro affinity assays showed that the recombinant fragment binds to the toxin, and mapped the binding site to the N-terminus of the receptor.
机译:昆虫病原芽孢杆菌是控制库蚊的一种重要工具,其有效性已在现场试验中得到验证。然而,对该细菌的抗药性的出现仍然对其使用构成威胁,并且已经尝试理解抗药性机制。先前的研究表明,在库克斯库克(Culex qu)inquefascia山雀菌落中对球形芽孢杆菌的抗性与幼虫中肠微绒毛中缺乏约60kDa的二元毒素受体有关。在这里,从易感菌落克隆并测序了编码西洋参线虫毒素受体Cqm1的基因。推导的氨基酸序列证实了其作为α-葡糖苷酶的身份,并且对来自抗性幼虫的相应基因序列的分析暗示了19个核苷酸的缺失作为抗性的基础。此删除会更改ORF,并产生一个过早的终止密码子,从而阻止了全长Cqm1的合成。但是,当用针对Cqm1的N端45 kDa重组片段的抗体探测整个幼虫提取物时,未检测到截短蛋白的表达。似乎过早的终止密码子将突变的cqm1引导到mRNA降解的无意义介导的衰变途径。凝胶内分析证实抗性菌落中缺少单个α-葡萄糖苷酶蛋白。进一步的体外亲和力测定表明重组片段与毒素结合,并将结合位点定位于受体的N-末端。

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