Hey everyone,
I'm working on creating a flow QC panel. I have a few sets of 3 intracellular and 3 surface markers that I know have worked well in the past for ICC and flow applications. My intracellular markers are all non-conjugated so I need to use secondary antibodies to put on the fluorochromes. I've titrated the initial unlabelled primary antibodies for the markers but I'm wondering if anybody sees the need to titrate the secondaries. Does anyone have some thoughts on this topic or should I just go with a 1:1000 dilution of them and wash a couple time to remove any unbound secondary?
Thanks,
Mike
Hi Mike,
I would say as long as you're confident with your unlabelled primary antibody titration, you're fine to go ahead with using a constant volume of secondary antibody. I would wash thoroughly with FACS buffer before/after staining and be ready to lose a few cells. From my experience, the first step is critical whilst the latter is less so. Good luck!
- Badges
- Science topic
- Similar topics
- Cognitive Science
- Thinking