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Using differential solubilization and 2-D gel electrophoresis to visualize increased numbers of proteins in the human cortex and caudate nucleus and putamen

机译:使用差异增溶和2-D凝胶电泳可视化人类皮层尾状核和壳状核中蛋白质数量的增加

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摘要

The aim of this study was to determine if differential solubilization of human CNS proteins would increase the total number of proteins that could be visualized using 2-D gel electrophoresis. Hence, proteins were solubilized into Tris, CHAPS and SB3–10 before separation across a pH 4–7 IEF gradient and a 12–14% SDS polyacrylamide gel, which could be achieved with a run-to-run variation of 35% in spot intensity. Because Western blot analyses suggested proteins could be in more than one detergent fraction, we completed a conservative analyses of our 2-D gels assuming spots that appeared on multiple gels at the same molecular weight and pI were the same protein. These analyses show that we had visualized over 3000 unique protein spots across three 2-D gels generated from each sample of human frontal cortex and caudate-putamen. This represented, at worst, a significant increase in the number of spots visualized in the acidic protein spectrum compared to what has been reported in other studies of human CNS. This study, therefore, supports the proposal that the analysis of the human CNS proteome using 2-D gel electrophoresis, combined with appropriate sample preparation, can be used to expand the studies on the pathologies of neurological and psychiatric diseases.
机译:这项研究的目的是确定人CNS蛋白的差异增溶是否会增加使用2-D凝胶电泳可以看到的蛋白总数。因此,在通过pH 4-7 IEF梯度和12-14%SDS聚丙烯酰胺凝胶进行分离之前,蛋白质先溶解为Tris,CHAPS和SB3-10,这可以通过点对点之间35%的连续变化来实现强度。由于蛋白质印迹分析表明蛋白质可能在一个以上的去污剂级分中,因此我们对二维凝胶进行了保守分析,假设在多个凝胶上以相同分子量和pI出现的斑点是相同蛋白质。这些分析表明,我们已经在每个人额叶皮层和尾状豆蔻样品中生成的三种2-D凝胶中观察到3000多个独特的蛋白质斑点。与其他有关人类中枢神经系统研究的报道相比,在最坏的情况下,这表示酸性蛋白质谱中可见斑点的数量显着增加。因此,本研究支持以下建议:使用2-D凝胶电泳结合适当的样品制备方法对人CNS蛋白质组进行分析,可用于扩大对神经和精神疾病病理学的研究。

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