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A strategy for enrichment of claudins based on their affinity to Clostridium perfringens enterotoxin

机译:一种基于claudins对产气荚膜梭菌肠毒素亲和力的富集策略

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Background Claudins, a family of protein localized in tight junctions, are essential for the control of paracellular permeation in epithelia and endothelia. The interaction of several claudins with Clostridium perfringens enterotoxin (CPE) has been exploited for an affinity-based enrichment of CPE-binding claudins from lysates of normal rat cholangiocytes.Results Immunoblotting and mass spectrometry (MS) experiments demonstrate strong enrichment of the CPE-binding claudins -3, -4 and -7, indicating specific association with glutathione-S-transferase (GST)-CPE_(116-319) fusion protein. In parallel, the co-elution of (non-CPE-binding) claudin-1 and claudin-5 was observed. The complete set of co-enriched proteins was identified by MS after electrophoretic separation. Relative mass spectrometric protein quantification with stable isotope labeling with amino acids in cell culture (SILAC) made it possible to discriminate specific binding from non-specific association to GST and/or matrix material.Conclusion CPE _(116-319) provides an efficient tool for single step enrichment of different claudins from cell lysates. Numerous proteins were shown to be co-enriched with the CPE-binding claudins, but there are no indications (except for claudins -1 and -5) for an association with tight junctions.
机译:背景claudins是位于紧密连接中的蛋白质家族,对于控制上皮和内皮中的细胞旁渗透至关重要。已开发了几种claudins与产气荚膜梭菌肠毒素(CPE)的相互作用,用于从正常大鼠胆管细胞裂解物中基于亲和力富集CPE结合claudins的结果。 claudins -3,-4和-7,表明与谷胱甘肽-S-转移酶(GST)-CPE_(116-319)融合蛋白有特定的关联。平行地,观察到(非CPE结合的)claudin-1和claudin-5的共洗脱。电泳分离后,通过质谱鉴定了完整的共富集蛋白。通过在细胞培养物中用氨基酸稳定同位素标记的相对质谱蛋白质定量(SILAC),可以区分特异性结合与GST和/或基质材料的非特异性结合。结论CPE_(116-319)提供了一种有效的工具用于从细胞裂解物中一步富集不同claudins。已显示许多蛋白质与结合CPE的claudins共富,但没有迹象表明(claudins -1和-5除外)与紧密连接有关。

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