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从电鳗电板膜中纯化与电压敏感性钠通道相关的河豚毒素结合成分。

Purification of the tetrodotoxin-binding component associated with the voltage-sensitive sodium channel from Electrophorus electricus electroplax membranes.

作者信息

Agnew W S, Levinson S R, Brabson J S, Raftery M A

出版信息

Proc Natl Acad Sci U S A. 1978 Jun;75(6):2606-10. doi: 10.1073/pnas.75.6.2606.

Abstract

The tetrodotoxin-binding component associated with the voltage-sensitive sodium channel from electroplax membranes of Electrophorus electricus has been purified. The toxin-binding site could be efficiently solubilized with Lubrol-PX, resulting in an extract of high initial specific activity. Purification was facilitated by the development of a rapid, quantitative binding assay. The binding component was stabilized during purification by the use of mixed lipid/detergent micelles of defined composition, and by the saturation of the site with tetrodotoxin. The purification was achieved by means of a highly selective adsorption of the toxin-binding component to DEASE-Sephadex A-25, followed by desorption at high ionic strength and chromatography over Sepharose 6B. Final peak specific activities were at least 50% of the specific activity expected for a pure, undenatured toxin-binding componenet of 230,000 molecular weight. The purified material exhibited a sedimentation coefficient of approximately 8 S and an unusual Stokes radius of 95 A. Purified material showed a relatively simple pattern on sodium dodecyl sulfate/polyacrylamide gel electrophoresis, being comprised of only three polypeptides.

摘要

与电鳗电板膜上电压敏感钠通道相关的河豚毒素结合成分已被纯化。该毒素结合位点可用Lubrol-PX有效溶解,从而得到具有高初始比活性的提取物。快速定量结合测定法的开发促进了纯化过程。在纯化过程中,通过使用特定组成的混合脂质/去污剂胶束以及用河豚毒素使位点饱和来稳定结合成分。通过使毒素结合成分高度选择性吸附到DEAE-葡聚糖凝胶A-25上,然后在高离子强度下解吸并在琼脂糖6B上进行层析来实现纯化。最终峰的比活性至少为预期分子量为230,000的纯的、未变性的毒素结合成分比活性的50%。纯化后的物质沉降系数约为8S,斯托克斯半径异常,为95埃。纯化后的物质在十二烷基硫酸钠/聚丙烯酰胺凝胶电泳上显示出相对简单的图谱,仅由三种多肽组成。

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