[Histonet] Re: double/triple staining with streptavidin-Alexa
C.M. van der Loos
c.m.vanderloos <@t> amc.uva.nl
Thu Mar 16 02:10:08 CST 2006
Dear Yves,
What Gayle Callis already mentioned about avidin-biotin blocking
before the first and the second sequence is indeed the only thing you
can do when combining two biotin techniques in double staining.
However, in general I don't recommend this for multiple staining. To
my opinion there is still a great risk for false positive results. As
Gayle described, the multistep procedure combining one unlabeled and
one biotinylated antibody works fine. I would like to add the option
of biotinylating or the labeling with an Alexa fluorochrome of one of
your primaries using the Zenon kit.
Good luck!
Chris van der Loos, PhD
Dept. of Pathology
Academic Medical Center M2-230
Meibergdreef 9
NL-1105 AZ Amsterdam
The Netherlands
phone: +31 20 5665631
Date: Tue, 14 Mar 2006 14:13:49 -0700
From: Gayle Callis <gcallis <@t> montana.edu>
Subject: Re: [Histonet] double/triple staining with streptavidin-Alexa
Fluor
To: Yves Heremans <Yves.Heremans <@t> vub.ac.be>,
Histonet <@t> lists.utsouthwestern.edu
Yes, however, using an avidin/biotin blocks before each antibody to
ensure
1) quenching endog biotin before first and quenching any residual
biotin
left over from first antibody sequence before you do the second
primary
sequence.
We do double IFA staining with two rat antimouse monoclonals in the
following way with one purified monoclonal and one biotinylated
monoclonal
primary.
Frozen sections fixed with acetone alcohol mixture at RT after
overnight drying
Normal serum block matched to host of secondary used
Strepavidin/biotin block (Vector)
Rat antiMouse monoclonal
Donkey antiRat F(ab')2 frag of IgG conjugated to RRX
Rat serum block, 5% for 15 minutes
Pri! mary #2 r
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