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Functional characterization of Musca glutamate- and GABA-gated chloride channels expressed independently and coexpressed in Xenopus oocytes

机译:在爪蟾卵母细胞中独立表达和共表达的Musca谷氨酸和GABA门控氯离子通道的功能表征

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Ligand-gated chloride channels (LGICs) are important targets for insecticides and parasiticides. Genes encoding subunits of two LGICs, a glutamate-gated chloride channel (MdGluCl-alpha) and a gamma-aminobutyric acid (GABA)-gated chloride channel (MdRdl), were cloned from house-flies (Musca domestica L.). These genes were first expressed independently in Xenopus laevis oocytes by cRNA injection in order to investigate the pharmacology of these ligand-gated channels using two-electrode voltage-clamp electrophysiology. It was found that L-glutamate and GABA activated the MdGluCl-alpha homo-oligomers with an EC(50) value of 30 microM and the MdRdl homo-oligomers with an EC(50) value of 101 microM, respectively. Both channels were chloride ion-permeable, and the MdRdl channel was more sensitive to chloride channel blockers, such as gamma-hexachlorocyclohexane (gamma-HCH), fipronil and picrotoxinin, than the MdGluCl-alpha channel. MdGluCl-alpha required only 1-2 days of incubation after cRNA injection to be expressed in oocytes, whereas 4-7 days of incubation was necessary to achieve MdRdl expression. However, when the cRNA of MdGluCl-alpha was injected at a dose of 1% (w/w) 1 day after the injection of the cRNA of MdRdl, a significant increase in the current amplitude of responses to GABA was observed, and the incubation period necessary for MdRdl expression became shorter. These results suggest that MdGluCl-alpha assists in the expression of MdRdl when the two are coexpressed.
机译:配体门控氯离子通道(LGIC)是杀虫剂和杀寄生虫剂的重要目标。从家蝇(Musca domestica L.)中克隆了编码两个LGICs的一个亚基的基因,一个谷氨酸门控的氯离子通道(MdGluCl-α)和一个γ-氨基丁酸(GABA)门控的氯离子通道(MdRdl)。这些基因首先通过cRNA注射在非洲爪蟾卵母细胞中独立表达,以便使用双电极电压钳电生理研究这些配体门控通道的药理作用。已发现,L-谷氨酸和GABA分别激活EC(50)值为30 microM的MdGluCl-α均聚物和EC(50)值为101 microM的MdRdl均聚物。这两个通道都是氯离子可渗透的,并且MdRdl通道比MdGluCl-α通道对氯离子通道阻滞剂(例如,γ-六氯环己烷(γ-HCH),氟虫腈和甲基毒素)更敏感。注射cRNA后,MdGluCl-alpha仅需要培养1-2天即可在卵母细胞中表达,而培养4-7天对于获得MdRdl表达是必需的。但是,当在注射MdRdl的cRNA后1天以1%(w / w)的剂量注射MdGluCl-α的cRNA时,观察到对GABA的当前反应幅度显着增加,并且孵育MdRdl表达所需的时间缩短。这些结果表明,当两者共表达时,MdGluCl-alpha有助于MdRdl的表达。

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