DAPI bleaching issue
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Hi list, One of my users has very quick DAPI bleaching when observing
her samples, wich sometimes make even difficult to get images. Most of my users
use routinely DAPI in their samples and never had such a problem. She is performing a immunofluorescence with the tyramide kit
from Perin Elmer (peroxidase blocking step, blocking with TNB, whashing steps
with TNT) on muscle mouse sections (10 µm thick approx). She is using Acetone
as a fixative (10 min), and is mounting with Vectashield after DAPI staining
(10 min). DAPI observation and imaging is performed on a Leica DM6000B
with a standard blue fluorescence filter and the Hg lamp set at minimum power
(10%). As I said, over the years tens of users have imaged DAPI staining on a
lot of different cells/tissues using the same setup and never observed such a
quick bleaching. Her protocol seems quite standard for me, but I have little experience
both with acetone as a fixative and with tyramide amplification, so perhaps I
am missing something. Also I have read in the list some issues with DAPI with
Vectashield. Any advice/tip will be welcome. Feel free to contact me off
list if you need the full protocol to make a better diagose. Thank you very much in advance! Best, ___________________________________
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How's her dye concentration compare to other users? Is there more oxygen around in the sample somehow? Is something wrong with the Vectashield prep?
Just some ideas we came up with 'around the water cooler'... Craig On Tue, Jan 20, 2009 at 4:50 AM, Xavier Sanjuan <[hidden email]> wrote:
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Lingle, Wilma L., Ph.D. |
Re: DAPI bleaching issue
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We have observed that after acetone or methanol fixation,
nuclei lose integrity over a relatively short period of time. Perhaps she
is observing that rather than photobleaching. We solved the problem by
doing a very short (para)formaldehyde fixation of the tissue on the slide after
immunolabeling and just prior to DAPI incubation.
Wilma Lingle
Wilma L. Lingle,
Ph.D. From: Confocal Microscopy List [mailto:[hidden email]] On Behalf Of Craig Brideau Sent: Tuesday, January 20, 2009 2:58 PM To: [hidden email] Subject: Re: DAPI bleaching issue Just some ideas we came up with 'around the water cooler'... Craig On Tue, Jan 20, 2009 at 4:50 AM, Xavier Sanjuan <[hidden email]>
wrote:
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Are you dual staining at all? I have had problems
with photobleaching of some probes when trying variable concentrations
of probe mixes. And have found that increasing concentrations of one
probe over another can cause a result of photobleaching of other probes in the
mix.
From: Confocal Microscopy List [mailto:[hidden email]] On Behalf Of Lingle, Wilma L., Ph.D. Sent: Wednesday, 21 January 2009 11:14 a.m. To: [hidden email] Subject: Re: DAPI bleaching issue We have observed that after acetone or methanol fixation,
nuclei lose integrity over a relatively short period of time. Perhaps she
is observing that rather than photobleaching. We solved the problem by
doing a very short (para)formaldehyde fixation of the tissue on the slide after
immunolabeling and just prior to DAPI incubation.
Wilma Lingle
Wilma L. Lingle,
Ph.D. From: Confocal Microscopy List [mailto:[hidden email]] On Behalf Of Craig Brideau Sent: Tuesday, January 20, 2009 2:58 PM To: [hidden email] Subject: Re: DAPI bleaching issue Just some ideas we came up with 'around the water cooler'... Craig On Tue, Jan 20, 2009 at 4:50 AM, Xavier Sanjuan <[hidden email]>
wrote:
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