[Histonet] HELP

[Connolly, Brett M]

We also use the MCA711 antibody (at 1.0 ug/mL, 1 hr.), but with HIER in citrate buffer using a Biocare Decloaker pressure cooker and Biocare's rat-on mouse HRP polymer detection. We  get very nice staining with no background. I was never too impressed with ImPRESS.

Here are the basics :
- Deparaffinize and hydrate to dH20
- Perform HIER, cool for 20 min then wash in H20
- 3.0% H2O2 - 20 min
- Serum free block (Biocare Sniper) 30 min
- Incubate with MCA771 1 hr.
- Incubate with Biocare rat-on-Mouse kit (per instructions)
- DAB - 5 min.
 Washes are with PBS/0.1% Tween

Brett


Brett M. Connolly, Ph.D.
Principle Scientist, Imaging Dept.
Merck & Co., Inc.
PO Box 4, WP-44K
West Point, PA 19486
brett_connolly <@t> merck.com
T- 215-652-2501
F- 215-993-6803




-----Original Message-----
From: histonet-bounces <@t> lists.utsouthwestern.edu [mailto:histonet-bounces <@t> lists.utsouthwestern.edu] On Behalf Of Elizabeth Chlipala
Sent: Thursday, November 06, 2014 12:41 PM
To: Hans B Snyder; histonet <@t> lists.utsouthwestern.edu
Subject: RE: [Histonet] HELP

Hans

We use the antibody from Serotec, it works quite nicely.  MCA711, proteinase K digestion,  rabbit anti-rat secondary and then Envision Rabbit (polymer).  We use this antibody at a 1:1200 dilution.

Liz

Elizabeth A. Chlipala, BS, HTL(ASCP)QIHC
Premier Laboratory, LLC
PO Box 18592
Boulder, CO 80308
(303) 682-3949 office
(303) 682-9060 fax
(303) 881-0763 cell
liz <@t> premierlab.com
www.premierlab.com

March 10, 2014 is Histotechnology Professionals Day

Ship to Address:

Premier Laboratory, LLC
1567 Skyway Drive, Unit E
Longmont, CO 80504


-----Original Message-----
From: histonet-bounces <@t> lists.utsouthwestern.edu [mailto:histonet-bounces <@t> lists.utsouthwestern.edu] On Behalf Of Hans B Snyder
Sent: Thursday, November 06, 2014 10:31 AM
To: histonet <@t> lists.utsouthwestern.edu
Subject: [Histonet] HELP

Hello All,

Does anyone have a protocol for the Anti-Neutrophil antibody [NIMP-R14]
(ab2557) for mouse tissue?  I have been trying to extinguish the background staining but cannot find the right combination.
​ We are doing this by hand. ​
 The recommended dilution for this antibody is 1:50 with HIER.   See used
protocol below.

So far I have tried:
1. concentrations 1:25, 1:50, 1:75, 1:100  - 1:50 gives very high background but good positive staining, 1:100 gives low background but not much positive staining.

2. HIER - 3, 5, 10,  20, minutes  @ 96C, 20 minutes at 60C  all give the same results - too much back ground

3. We have tried using the H2O2 before the primary and after, increasing the time from 30 minutes to 45 minutes.

4. Tried incubating in the primary for shorter time (20 minutes) and longer overnight at 4C.

5. Tried blocking using 3 different serums, first each one then combinations and longer times.

6. Tried cutting the DAB concentration in 1/2 then 1/3.


We have not tried enzyme or acid epitope retrieval yet.



*Does anyone have a working protocol or suggestions on what to try?*


​Thank you in advance.​





Procedure:

Deparaffinize

1.      Heat slides to 60C for 10 minutes (oven).

2.      Dry slides at room temp 5 minutes.

3.      Xylene 5 minutes.

4.      Xylene 5 minutes.

5.      100% ethanol 5 minutes (dehydration).

6.      100% ethanol 2 minutes (dehydration).

7.      95% ethanol for 2 minutes (rehydration).

8.      70% ethanol for 2 minutes (rehydration).

9.       Run in DI water for 10 minutes.



Antigen Retrieval

1.      Submerge in 0.01M Citrate Buffer (pH 6.0) at 96C for 5 minutes.

2.      Cold running water 5 minutes.



Staining

1.      Wash in PBS for 1 min.

2.      Permeabilize with 0.1% Triton X / 2.5% horse serum + 2.5% fetal
bovine serum for 2 hours.

3.      Incubate in primary antibody 30-45 minutes at in 2.5% horse serum
in PBS.

4.      Wash 3x in PBS/tween for 5 minutes each.

5.      Fresh 3.0% hydrogen peroxide (H2O2) 2x for 20 minutes each.

6.      Wash 3x PBS 2 minutes each.

7.      Incubate with anti-Rat Ig impress solution (according to vector’s
instructions) 45 minutes.

8.      Wash 3x in PBS for 5 minutes each.

9.      Prepare Impact DAB substrate (see insert).

10.  Using a light microscope, incubate sections with 50-100ul, until desired darkness occurs (5-30 seconds).

11.  Stop DAB reaction using deionized water.

12.  Wash in DH2O for 5 minutes

13.  Counterstain in Harris hematoxylin for 30 seconds.

14.  Wash in DH2O for 5 minutes.

15.  Dehydrate 2x in 95% alcohol for 30 seconds each.

16.  Dehydrate 3x in 100% alcohol for 2 minutes each.

17.  Clear 2x in xylene 5 minutes each.

18.  Mount coverslips using Leica mounting media.


Hans B Snyder
Histologistics
60 Prescott Street
Worcester, MA 01605
508-308-7800
hans <@t> histologistics.com
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