BrdU Staining

Paul Zimmer (Paul.Zimmer@ccc.uab.edu)
Thu, 27 Feb 1997 16:11:48 -0600

Messages sorted by: [ date ][ thread ][ subject ][ author ]
Next message: Frederick Garbrecht: "Re: Pipettors for Terasaki Plates"
Previous message: Joseph Webster: "Re: absolute counts - a side issue"

Our laboratory has been using the standard acid-denaturation protocol
for testing BrdU incorporation by flow, but we have been disappointed by
the number of common epitopes destroyed during this process (e.g. CD23
on murine B-cells). We have been testing the DNAse protocol described
by John Sprent's group, but with little success. All of the key
reagents were recently purchased and work well in other assays. I am
curious about two aspects of the protocol:

1) Does azide interfere with the DNAse enzyme activity? (we use azide in
our common stock of 1% paraformaldehyde solution)

2) Does the source of DNAse make a difference? (we have been using
molecular biology grade RNAse-free DNAse I)

Any other suggestions or helpful comments on common problems would be
greatly appreciated. We have already spoken with Dr. Sprent's lab and
they have not had similar problems.

--------
J. Paul Zimmer, Ph.D.
Developmental and Clinical Immunology
University of Alabama at Birmingham

Next message: Frederick Garbrecht: "Re: Pipettors for Terasaki Plates"
Previous message: Joseph Webster: "Re: absolute counts - a side issue"