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Use of a purified and functional recombinant calcium-channel beta4 subunit in surface-plasmon resonance studies.

机译:纯化和功能重组钙通道β4亚基在表面等离子体共振研究中的用途。

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摘要

Native high-voltage-gated calcium channels are multi-subunit complexes comprising a pore-forming subunit Ca(v) and at least two auxiliary subunits alpha(2)delta and beta. The beta subunit facilitates cell-surface expression of the channel and contributes significantly to its biophysical properties. In spite of its importance, detailed structural and functional studies are hampered by the limited availability of native beta subunit. Here, we report the purification of a recombinant calcium-channel beta(4) subunit from bacterial extracts by using a polyhistidine tag. The purified protein is fully functional since it binds on the alpha1 interaction domain, its main Ca(v)-binding site, and regulates the activity of P/Q calcium channel expressed in Xenopus oocytes in a similar way to the beta(4) subunit produced by cRNA injection. We took advantage of the functionality of the purified material to (i) develop an efficient surface-plasmon resonance assay of the interaction between two calcium channel subunits and (ii) measure, for the first time, the affinity of the recombinant His-beta(4) subunit for the full-length Ca(v)2.1 channel. The availability of this purified material and the development of a surface-plasmon resonance assay opens two immediate research perspectives: (i) drug screening programmes applied to the Ca(v)/beta interaction and (ii) crystallographic studies of the calcium-channel beta(4) subunit.
机译:天然高压门控钙通道是多亚基复合物,包括孔形成亚基Ca(v)和至少两个辅助亚基α(2)δ和β。 β亚基可促进通道的细胞表面表达,并对其生物物理特性有重要贡献。尽管它很重要,但是由于天然β亚基的有限可用性而无法进行详细的结构和功能研究。在这里,我们报告通过使用多组氨酸标签从细菌提取物中纯化重组钙通道β(4)亚基。纯化的蛋白质是完全功能性的,因为它结合在alpha1相互作用域上,是其主要的Ca(v)结合位点,并以与beta(4)亚基相似的方式调节非洲爪蟾卵母细胞中表达的P / Q钙通道的活性。通过cRNA注射产生。我们利用纯化材料的功能来(i)开发两个钙通道亚基之间相互作用的有效表面等离子体共振测定,并且(ii)首次测量了重组His-beta( 4)全长Ca(v)2.1通道的亚基。这种纯化材料的可用性和表面等离子体共振分析的发展打开了两个直接的研究视角:(i)适用于Ca(v)/β相互作用的药物筛选程序,以及(ii)钙通道β的晶体学研究(4)亚单位。

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