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Binding of murine monoclonal antibodies to the active and inactive configurations of aequorin

机译:鼠单克隆抗体与水母发光蛋白的活性和非活性构型的结合

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摘要

>Murine monoclonal IgG1 antibodies (MAb), designated Aq-11 and Aq-12, were prepared against the photoprotein aequorin from jelly fish. Aequorin is a calcium-sensitive photoprotein which consists of a single polypeptide chain, apoaequorin, and a functional chromophore, coelenterazine. Native aequorin consists of two species with molecular masses of 25 and 23.5 kDa. MAb Aq-12 was found by immunoblot analysis to bind specifically to the 25 kDa species, while MAb Aq-11 reacted with the 23.5 kDa protein. Activation of apoaequorin with coelenterazine was associated with a shift of the 23.5 kDa molecule to the 25 kDa species. In contrast, treatment with calcium ions induced a shift back to the 23.5 kDa form. These changes between the active and inactive forms were identified by reactivity with MAbs Aq-11 and Aq-12. The results thus indicate that these MAbs should be useful in monitoring activation of this photoprotein.
机译:制备了针对水母光蛋白水母发光蛋白的>鼠单克隆IgG 1 抗体(MAb),称为Aq-11和Aq-12。水母发光蛋白是对钙敏感的光蛋白,它由一条多肽链载水母发光蛋白和功能发色团腔肠素组成。天然水母发光蛋白由分子量为25和23.5 kDa的两个物种组成。通过免疫印迹分析发现MAb Aq-12与25 kDa物种特异性结合,而MAb Aq-11与23.5 kDa蛋白反应。用腔肠素激活载水母发光蛋白与将23.5 kDa分子转移到25 kDa物种有关。相比之下,用钙离子处理可导致移回到23.5 kDa形式。通过与单克隆抗体Aq-11和Aq-12的反应来鉴定活性形式和非活性形式之间的这些变化。因此,结果表明这些MAb应可用于监测该光蛋白的活化。

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