(no subject)

Hi List,

One of my colleagues is trying to visualize a nuclear protein using primary antibodies. Is there a special trick  or protocol that allows the primary and the fluorescent secondary antibodies better access to proteins inside the nucleus? They have already considered using either Triton or Tween-20.

Thanks,

Neeraj.

Neeraj V. Gohad, Ph.D.

Postdoctoral Fellow

Okeanos Research Group

Department of Biological Sciences

132 Long Hall

Clemson University

Clemson,SC-29634

Phone: 864-656-3597

Fax: 864-656-0435

Please note my new email address: [hidden email]

Hi List,

One of my colleagues is trying to visualize a nuclear protein using primary antibodies. Is there a special trick  or protocol that allows the primary and the fluorescent secondary antibodies better access to proteins inside the nucleus? They have already considered using either Triton or Tween-20.

Thanks,

Neeraj.

Neeraj V. Gohad, Ph.D.

Postdoctoral Fellow

Okeanos Research Group

Department of Biological Sciences

132 Long Hall

Clemson University

Clemson,SC-29634

Phone: 864-656-3597

Fax: 864-656-0435

Please note my new email address: [hidden email]

Danielle Crippen

Morphology and Imaging Core

Hi List,

One of my colleagues is trying to visualize a nuclear protein using primary antibodies. Is there a special trick  or protocol that allows the primary and the fluorescent secondary antibodies better access to proteins inside the nucleus? They have already considered using either Triton or Tween-20.

Thanks,

Neeraj.

Neeraj V. Gohad, Ph.D.

Postdoctoral Fellow

Okeanos Research Group

Department of Biological Sciences

132 Long Hall

Clemson University

Clemson,SC-29634

Phone: 864-656-3597

Fax: 864-656-0435

Please note my new email address: [hidden email]

Hi Mario,

This is a new project for my colleague, they have tried using a standard fixation protocol (4% buffered PFA, 0.5% Triton, block with BSA etc..) to no avail.

Best,

Neeraj.

Hi List,

One of my colleagues is trying to visualize a nuclear protein using primary antibodies. Is there a special trick  or protocol that allows the primary and the fluorescent secondary antibodies better access to proteins inside the nucleus? They have already considered using either Triton or Tween-20.

Thanks,

Neeraj.

Neeraj V. Gohad, Ph.D.

Postdoctoral Fellow

Okeanos Research Group

Department of Biological Sciences

132 Long Hall

Clemson University

Clemson,SC-29634

Phone: 864-656-3597

Fax: 864-656-0435

Please note my new email address: [hidden email]

--

Many Thanks to everyone who replied to my staining of nuclear proteins post. I have compiled the suggestions and protocols of the folks who replied.

Best Regards and have a Good Weekend!

Neeraj.

Neeraj V. Gohad, Ph.D.

Postdoctoral Fellow

Okeanos Research Group

Department of Biological Sciences

132 Long Hall

Clemson University

Clemson,SC-29634

Phone: 864-656-3597

Fax: 864-656-0435

Please note my new email address: [hidden email]

1)    The fixation, not membrane permeabilization, seems to be more of a factor for nuclear proteins.

            Try Methanol (100% formaldehyde-free at -20C for 20 min). Compare with 3.7% FA at RT.

            Contact me off-list if you need further details.

            Besrt Wishes,

           Fred E. Indig, Ph.D.

           Head, Confocal Imaging Facility

2)    You don't mention the fixation protocol used. If and when to use Triton (0.2-0.5%; harsh) or Tween (gentler) in part depends on the fixation protocol. Staining nuclear proteins presents its own problems aside from simply permeabilizing the membrane barriers that let your antibodies in. Non-specific labeling is often greatly enhanced because of local ionic strength, pH and very strong electrostatic interactions. You could have a very high affinity antibody (primary and/or secondary) and still end up with diffuse (as in worthless) staining.

Cold methanol/acetone fixation might be the way to go if PFA (2-3%) plus Triton (0.5%) doesn't seem to work. Also, staining using higher ionic strength can be helpful and consider conjugating a fluorophore to your primary and forget the secondary altogether. How you block your cells can also be very important.

Mario

3)    I used to have pretty good success accessing DNA binding proteins using 0.5% triton for about 15minutes.Cold MetOH fixation also worked well...

            Good luck!

 Danielle Crippen

Morphology and Imaging Core Manager

Buck Institute for Age Research

4)    Can you define failure? No staining, gross non-specific staining, lack of expected labeling morphology? If you don't get any signal then the antibodies are probably not working. Try new antibodies. In the nucleus the antibody might be unable to "find" its target epitope. It might be comprised through binding to the high concentrations of nucleic acid, matrix proteins, etc. Labeling at elevated temperature might help

(37°C) or playing with the pH and elevated ionic strength or staining for a long time (overnight in the refrigerator). But it does depend on what you mean by failure. BTW, I have never found BSA to be a very good blocker, but that is a specificity issue not an invisibility one. Stickiness inside the nucleus translates into a reduced rate of diffusion. To a first order, the diffusion constant of a large protein will decrease in proportion to the apparent partitioning coefficient of the protein to the sticky environment it interacts with and depends on the antibody's charge, etc. So something that would normally label in 15 minutes could take a few hours at rm. temperature.

Mario

5)    Did they do a concentration curve of their primary Ab? Even if working in WB, if used at the same concentration, it will probably be the wrong concentration... I have been using the following protocol with very consistent results in confocal:
- PAF 4%, 5 min RT
- rinse in PBS 3x 5 min in rotation (cells on coverslips in 6 wells plate)
- block in PBS/Triton X100 0.2% (tx)/normal serum 10% (NS) (goat if secondary is from goat) for 15 min in rotation
- primary Ab for 1 hr in PBS/Tx/NS at RT (or at 4 degree C overnight), in rotation
- rinse in PBS 2x5 min in rotation
- block in PBS/Tx/NS 15 min in rotation
- secondary Ab 1 hr in PBS/Tx/NS at RT
- rinse in PBS
- rapid wash in tap water prior to mounting.
Hope this will help.

Best,

Myriam

6)    Comment posted on behalf of a colleague (Prasanna Kumar) with considerable experience in staining nuclear proteins:

The protocol you use depends on the localization of the protein of interest in nucleus (found in  nucleoplasm or a DNA binding etc.) In general I found both Methanol and 4%FA protocols are good enough for most of the proteins with FA protocol maintaining the integrity of DNA/Nucleus better than Methanol.  Simultaneous Fixation( with3.7%FA,4%sucrose) and Permeabilization with 1%Triton X seemed to work well for DNA bound proteins and also different histone modifications. One thing is sure, with the nuclear proteins you need to try all these methods and compare the results as sometimes you see redistribution of the whole pattern and will be wondering which one is the true representative. Good Luck.

Barry O'Brien

7)    In our experience, the critical point in staining nuclear proteins is to facilitate antibody access to relevant epitopes. You can increase access by extending the incubations times with primary antibody (24 hours and beyond, at room temp.), using Fab fragments (~50kDa) instead of whole antibody molecules (~150kDa for IgGs) or, if you are interested exclusively in the stain of the nucleus, trying controlled permeabilizations of the cells with saponin or digitonin (mild

detergents) before fixation.

We favoured PFA fixation (2%) over cold methanol or acetone, which tends to collapse cell structures to a higher extent. There is a paper - 19751214[PMID] - with the details of our recent struggles to stain a protein in the nucleus. As a control, we expressed GFP, which localizes within nuclei, and compared the direct (green) fluorescence with the indirect (Vg. red) fluorescence obtained by immunocytochemistry.

Hope it helps

F Javier Díez Guerra, PhD

Profesor Titular