丙烯酰胺
堆积
色谱法
聚丙烯酰胺凝胶电泳
化学
特里斯
聚丙烯酰胺
电泳
缓冲器(光纤)
反离子
毛细管电泳
离子
高分子化学
生物化学
有机化学
聚合物
电信
计算机科学
共聚物
酶
作者
I. Piotr Maly,Cordula Nitsch
标识
DOI:10.1002/elps.200600688
摘要
In the attempt to separate in a single gel run low- and high-molecular-weight proteins, we present here a multiphasic buffer system designed for this purpose. It avoids the continuous stacking of SDS as it occurs in the 'classical' SDS-PAGE. The system allows complete stacking and destacking of proteins in the 3.5-250 kDa range at acrylamide concentrations as low as 4.5% T (total acrylamide concentration in %) and 2.6% C (degree of cross-linking in %). Taurine is used as the trailing ion in the cathode buffer and in the resolving zone of the gel, and two different counterions (Tris and imidazole) in the stacking zone. The gel system is easy to prepare and, due to the very low acrylamide concentrations, it is ideal for analytical as well as for preparative tasks.
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