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A gel-based method for purification of apolipoprotein A-I from small volumes of plasma

机译:从少量血浆中纯化载脂蛋白A-I的基于凝胶的方法

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摘要

We present here a gel-based method for rapid purification of apolipoprotein A-I (apoA-I) from small volumes of human plasma. After isolation of high density lipoprotein from plasma, the apoA-I protein was separated by electrophoresis and the apoA-I band excised from the gel. The apoA-I was then eluted from the gel strip, concentrated, and delipidated ready for use. The structure and function of the gel-purified apoA-I protein was compared against apoA-I purified by the traditional size-exclusion chromatography method. The α-helical content of the gel-purified apoA-I as determined by circular dichroism was similar to chromatography-purified apoA-I. The functional activity of gel-purified apoA-I, as determined by cholesterol efflux assays in primary human fibroblasts and RAW264.7 macrophages, was also comparable with chromatography-purified apoA-I. This method is a valid alternative for apoA-I purification with some advantages over traditional chromatography purification including a much reduced plasma volume requirement, less time and cost, and a higher percentage protein recovery. The method is particularly suitable for applications requiring the purification of apoA-I from multiple human or animal samples of interest.
机译:我们在这里介绍一种基于凝胶的方法,可从少量人血浆中快速纯化载脂蛋白A-I(apoA-I)。从血浆中分离出高密度脂蛋白后,通过电泳分离apoA-I蛋白,并从凝胶上切下apoA-I条带。然后从凝胶条上洗脱apoA-I,浓缩并脱脂以备使用。将凝胶纯化的apoA-I蛋白的结构和功能与通过传统尺寸排阻色谱法纯化的apoA-I进行了比较。通过圆二色性测定的凝胶纯化的apoA-I的α-螺旋含量类似于色谱纯化的apoA-I。通过在原代人成纤维细胞和RAW264.7巨噬细胞中通过胆固醇外流测定确定的凝胶纯化的apoA-I的功能活性也与色谱纯化的apoA-I相当。该方法是apoA-I纯化的有效替代方法,具有优于传统色谱纯化的一些优势,包括大大减少的血浆体积要求,更少的时间和成本以及更高的蛋白质回收率。该方法特别适用于需要从多个目标人类或动物样品中纯化apoA-1的应用。

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