I need to compare level of expression of a protein in E.coli cell lysates. In order to do so we want of take equal amount of protein from cell lysates. But I have too many samples to be processed by biochemical assays like Bradford etc.

We ended up normalizing the UV280 absorbance of all samples by fixing the absorbance at UV280 to 0.5.

My query is regarding the usage of using same UV280 as a measure of protein amounts to be loaded for western. Has anyone been following the practice?

More Himanshu Sharma's questions See All
Similar questions and discussions