As the title suggests, should SDS and/or methanol be included in the transfer buffer for transferring large molecular weight proteins (>300 kDa)? If so, how much of each is optimal?
For context, I am using 3-8% Tris-Acetate gels and transferring to 0.45uM nitrocellulose membranes overnight at 4degC.
Tomasz Fraczyk
If you want to preserve the native conformation of a protein you should rather avoid SDS for the transfer. I have done transfer without SDS and it worked pretty well. I am not sure about methanol, but I think you can/should avoid it as well.
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