RE: Hoechst vs FITC: possible?

kukuruga%kasle1.dnet.wayne.edu@rocdec.roc.wayne.edu
Thu, 8 Feb 1996 09:59:02 -0500

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Previous message: Howard Shapiro: "Re: Hoechst vs FITC: possible?"

H33342 with FITC is only possible, I believe, with a"time" displaced
signal. If you run a fluorescence spectrum on H33342, you will find a
relatively complex emmission profile, with significant fluorecence
at 530nm. This is also more problematic due to the variabliity of
absorption/emmission with time of staining and concentration of the
dye. If you need to acquire these parameters colinearily, use a
Red-shifted dye, like 7-AAD.
I routinely use H33342 at approx. 10 uM. I have tried to go as low
as 5 uM and lost stoichiometry. This was in viable L1210 cells --
these cells were sensitive to H33342 at 10 um, but 5 uM was
inadequate for labeling. For fixed cells, it's important to note
that dye accessibility is improved to the extent of requiring at
least a 10x dilution of the H33342 -- perhaps more (needs to be tested).

Next message: kukuruga%kasle1.dnet.wayne.edu@rocdec.roc.wayne.edu: "Re: Hoechst vs FITC: possible?"
Previous message: Howard Shapiro: "Re: Hoechst vs FITC: possible?"

CD ROM Vol 2 was produced by staff at the Purdue University Cytometry Laboratories and distributed free of charge as an educational service to the cytometry community. If you have any comments please direct them to Dr. J. Paul Robinson, Professor & Director, PUCL, Purdue University, West Lafayette, IN 47907. Phone:(317) 494-0757; FAX (317) 494-0517; Web http://www.cyto.purdue.edu EMAIL robinson@flowcyt.cyto.purdue.edu