Brett

Safranin O can be a bit tricky at times.   There are a few tips that we have 
used through the years.

1.  Fresh reagents are key.
2.  For proteoglycan staining you can cut the sections a bit thicker and get 
better staining we typically cut the joint sections for Saf O at 6 to 7 microns 
in thickness, there are papers out there that recommend up to 8 microns in 
thickness.
3.  Limit excess time in decal for some reason this particular stain may not 
work as well if the samples are in decal for an extended period of time, we 
have not seen this with toluidine blue which is another stain for proteoglycan.
4.  We increase times in the safranin O reagent on occasion for the murine 
joints.

Good Luck

Liz

Elizabeth A. Chlipala, BS, HTL(ASCP)QIHC
Laboratory Manager
Premier Laboratory, LLC
PO Box 18592
Boulder, CO 80308
Work (303) 682-3949
Fax (303) 682-9060
Cell (303) 881-0763
l...@premierlab.com
www.premierlab.com

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-----Original Message-----
From: histonet-boun...@lists.utsouthwestern.edu 
[mailto:histonet-boun...@lists.utsouthwestern.edu] On Behalf Of Brett Tonkin
Sent: Tuesday, May 21, 2013 11:08 PM
To: histonet@lists.utsouthwestern.edu
Subject: [Histonet] Safranin O cartilage staining

Hi,

We're having trouble staining murine articular cartilage with Safranin O. We 
first started using this stain last year and it was working nicely, with strong 
staining of both the articular cartilage and growth plate. After a while, the 
stain stopped working, with staining only visible in the growth plate. We 
replaced all solutions (including c/stain of fast green) and the staining 
worked. Yet again, it has stopped working, and this is only the second time the 
solutions have been used.

Has anyone come across this before?

Any help or advice would be greatly appreciated!


Brett Tonkin

Research Assistant
Arthritis Research Laboratory
Bone Cell Biology and Disease Unit
St. Vincent's Institute
Fitzroy, Victoria


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