A simple method of electroelution of individual protein bands from SDS polyacrylamide gels for direct study in cellular assays.

Journal of immunoassay Pub Date : 2000-11-01 DOI:10.1080/01971520009349542

S Bhaskar, S Dutt, R Mukherjee

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引用次数: 11

Abstract

A very simple and effective procedure which allows simultaneous electroelution of separated proteins from SDS polyacrylamide gel into small quantity of elution buffer is described. Elution parameters have been optimized for maximum possible recovery (50-60%). Protein fractions were collected in physiological buffer and an efficient removal of SDS have been obtained, thus fractions collected were suited for direct testing in cell cultures. Method was used to investigate human T-cell responses to purified secreted M tuberculosis H37Rv proteins. Eight low molecular weight (M.w. range 10 kD to 25 kD) culture filtrate proteins were purified in quantities, sufficient for immunological characterization. Lymphocyte proliferative responses and cytokine release pattern from tuberculosis patients, healthy contacts and healthy controls were studied on stimulation with purified culture filtrate proteins. Immunologically important M.tuberculosis proteins were identified by using this method. This approach should be applicable to the rapid identification and characterization of any interesting T cell antigen.

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一种简单的从SDS聚丙烯酰胺凝胶中电洗脱单个蛋白带的方法，用于细胞分析的直接研究。

一个非常简单和有效的程序，允许同时电洗脱分离的蛋白质从SDS聚丙烯酰胺凝胶到少量洗脱缓冲液描述。优化了洗脱参数，以获得最大可能的回收率(50-60%)。在生理缓冲液中收集蛋白质组分，获得了SDS的有效去除，因此收集的组分适合于在细胞培养中直接测试。方法观察人t细胞对纯化分泌结核分枝杆菌H37Rv蛋白的反应。8个低分子量(分子量范围为10 ~ 25 kD)的培养滤液蛋白被大量纯化，足以用于免疫学鉴定。研究了纯化培养滤液蛋白刺激肺结核患者、健康接触者和健康对照的淋巴细胞增殖反应和细胞因子释放模式。用这种方法鉴定了具有重要免疫学意义的结核分枝杆菌蛋白。这种方法应该适用于任何感兴趣的T细胞抗原的快速鉴定和表征。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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Journal of immunoassay

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