细胞分离
胞浆
分馏
U937电池
亚细胞定位
蛋白质亚细胞定位预测
细胞器
溶解
等密度
细胞生物学
化学
膜
密度梯度
内质网
生物化学
生物
色谱法
细胞
差速离心
细胞质
离心
细胞培养
酶
基因
物理
量子力学
遗传学
作者
William D. McCaig,Timothy J. LaRocca
摘要
This protocol describes a method to obtain subcellular protein fractions from mammalian cells using a combination of detergents, mechanical lysis, and isopycnic density gradient centrifugation. The major advantage of this procedure is that it does not rely on the sole use of solubilizing detergents to obtain subcellular fractions. This makes it possible to separate the plasma membrane from other membrane-bound organelles of the cell. This procedure will facilitate the determination of protein localization in cells with a reproducible, scalable, and selective method. This method has been successfully used to isolate cytosolic, nuclear, mitochondrial, and plasma membrane proteins from the human monocyte cell line, U937. Although optimized for this cell line, this procedure may serve as a suitable starting point for the subcellular fractionation of other cell lines. Potential pitfalls of the procedure and how to avoid them are discussed as are alterations that may need to be considered for other cell lines.
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