I am currently using Native agarose gel electrophoresis to discriminate between 3 proteins of a different pI, so my running buffer is Tris-glycine (pH 8.5). Could you please suggest a running buffer of a different pH (preferably close to 6-7)?
Thank you all in advance
It is important that the buffer system used has a low ionic strength, which allows the moving front build up a strong electrical field behind it. Bis-Tris is a good choice for this; but as Adron Ung , I have not personally used it.
Have you searched the literature? It is a while ago that I did my PhD, but I had - unfortunately no longer - a large collection of different electrophoresis recipes, all easily found in the literature. You could also check the websites of electrophoresis equipment manufacturers. GE has swallowed over the last 2 decades several companies that were once strong in this field; perhaps they still provide corresponding information on their site.
May I ask, why are you using agarose and not polyacrylamide?
Are your proteins so large?
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