It's a good idea to have "positive control" conditions with the cells you are using.

For a damage condition, I rather recommend DNA damaging chemicals because it is much easier to control than UV light in the hood which you have not calibrated.

Phleomycin from InvivoGen, for example, is not too expensive. Our student detected very clear increase of gamma-H2AX after 2 hr treatment with 100 µg/ml Phleomycin in several cell lines.

Shin-Ichiro Hiraga Thank you for your advice, I will look into Phleomycin. Could you tell me how the gamma H2AX was detected? Did you use WB and if yes could you let me know gel types, %, run and transfer conditions please?

Hi,

Here are the answers to your questions:

- We use Cell Signaling Technology #9718 gamma H2AX antibody, but I believe your antibody is also good.

- Yes, we are doing western blot

- Either 4-15% or 4-20% TGX gels from Bio-Rad are used, usually Stain-Free

- We use Bio-Rad Turbo Transfer (semi-dry with proprietary transfer buffer) system with "mixed MW" condition

- We use H2A.X antibody (Abcam ab11175) as a loading control.

I hope this helps.

Shin-Ichiro Hiraga Thanks for the details, I already used the same 4-15% BioRad gel so at least I can cross that off the list of potential problems with my protocol. I'm not aware of the transfer system you mention, I currently use a wet transfer tank from BioRad. I'll keep troubleshooting.