I am trying to run an SDS-PAGE gel 12% for p53 and alpha-actin and running into some trouble. I am using tissue samples that were fixed with PFA and this is likely the cause of the issues I'm having. BCA assay does not work, likely because of protein cross-linking due to PFA so I have to do a western for actin to get protein concentration, however even after boiling the samples and using SDS as well as BME I get no bands at all or weak bands.

In many membranes I see protein aggregates at the transition from the stacking to resolving gel and think this is a migration issue due to PFA cross-linking and creating protein aggregates. I am boiling my samples for 10 minutes, thinking of increasing this or doing a commassie stain to look for abnormal migration.

What does everyone think? Any experience with this? Suggestions?

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