I read the paper of Nauta with great interest!

But I dont have the original pdf for the paper on Stain Technology in 1951 & 
1954. Anyone can send me the pdf?

I only have the improved method by Fink and Heimer in 1967 published on brain 
research, giving out two staining procedures. I can send you the pdf if anyone 
is interested in this.

I would like to receive any proved protocol of silver staining for degenerating 
axons...because we dont have uranyl nitrate or hydroquinone  here...I can not 
repeat the paper by Fink & Heimer. 

Can anyone provide me a supressive procedure in staining degenerating axons 
using "common chemicals", just ammonia water, silver nitrate, citric acid, 
formalin/PFA, sodium hydroxide? I just can not find applicable one with our 
current facilities!

Thanks very much!


2008-12-15 



tf 



发件人: John Kiernan 
发送时间: 2008-12-15  13:42:09 
收件人: Susan Bachus 
抄送: Pat Flannery; Weems, Joyce; histonet 
主题: Silver & ammonia (Was Re: [Histonet] Silly Question? , , ,) 
 
Dear Susan,
Thank you for bringing Walle Nauta's 1993 review article to Histonetters' 
attention. I hadn't seen it before, and I agree that it was well worth 
downloading, reading and filing for future reference. 
More than 50 years ago Nauta & Gygax published a very easily understood account 
of ammoniacal silver solutions and the effects of changing their pH. This is 
fundamental to all techniques involving silver nitrate and ammonia, and the 
exact information is not in chemistry textbooks. Here's the reference.
Nauta WJH, Gygax PA (1951) Silver impregnation of degenerating axon terminals 
in the central nervous system: (1) Technic. (2) Chemical notes. Stain 
Technology 26: 5-11. 
Part 2 was an appendix to their paper on the early (non-suppressive) 
Nauta-Gygax method, which stains both normal and degenerating axons. Many of 
the principles explained in Part 2 of this paper apply also to other silver 
methods. 
If your library subscribes to journals published by Informa, you can download 
this Nauta-Gygax paper (and anything else in Stain Technology) as a PDF file 
from the InformaWorld web site: 
http://www.informaworld.com/smpp/title~content=t713692932~bb=all
The journal's name shows on the present publisher's web site in its present 
form (Biotechnic & Histochemistry) even though the name was really Stain 
Technology before about 1990. 
This is a problem with quite a few journals that have changed their names. The 
Springer web site, for example, doesn't seem to recognize the name changes of 
Histochemie --> Histochemistry --> Histochemistry and Cell Biology. Library 
catalogues usually record name changes faithfully.  For journals, changing the 
name probably isn't always a good move!
John Kiernan
Anatomy, UWO
London, Canada
= = =
----- Original Message -----
From: Susan Bachus <susanbac...@verizon.net>
Date: Friday, December 12, 2008 20:33
Subject: Re: [Histonet] Silly Question? - Need help quickly!
To: rjbu...@yahoo.com, Pat Flannery <pjfne...@duke.edu>, 
histonet@lists.utsouthwestern.edu, "Weems, Joyce" <jwe...@sjha.org>
> I tried earlier to send, for this thread, a wonderful paper by 
> Nauta, 
> chronicaling the history his discovery of his tract tracing 
> method, in which 
> serendipity and degradation of formalin played critical roles, 
> not realizing 
> that the size of the attachment would prevent it from going 
> through, so I am 
> trying again with a URL for this paper:
> http://www.jneurosci.org/cgi/reprint/13/4/1337
> 
> Susan
> 
> ----- Original Message ----- 
> From: "Rene J Buesa" <rjbu...@yahoo.com>
> To: "Pat Flannery" <pjfne...@duke.edu>; 
> <histonet@lists.utsouthwestern.edu>; 
> "Weems, Joyce" <jwe...@sjha.org>
> Sent: Thursday, December 11, 2008 12:58 PM
> Subject: RE: [Histonet] Silly Question? - Need help quickly!
> 
> 
> Joyce:
> Methanal, which is the chemical name of formaldehyde, 
> polymerizes. If it 
> forms a polymer of at least 50 molecules or more, it gets solid 
> = 
> para-formaldehyde.
> Formalin (a trade name as formol is also another trade name)is 
> the 37-50% 
> aqueous solution of formaldehyde (with some additiveses to 
> prevent 
> polymerization).
> You can prepare BNF using the formalin solution or dissolving 
> the amount of 
> solid para-formaldehydede to get to the concentrationon you desire.
> The chemical in both solutions is the same = methanal or 
> formaldehyde.Ren?
> J.
> 
> --- On Thu, 12/11/08, Weems, Joyce <jwe...@sjha.org> wrote:
> 
> 
> From: Weems, Joyce <jwe...@sjha.org>
> Subject: RE: [Histonet] Silly Question? - Need help quickly!
> To: "Pat Flannery" <pjfne...@duke.edu>, 
> histo...@lists.utsouthwestern.edudate: Thursday, December 11, 
> 2008, 12:12 PM
> 
> I was just going to post a question regarding paraformaldhyde myself!
> Just last week I believe I remember someone saying that 
> paraformaldehydeand formalin are the same and they had put the 
> same solution in two
> different containers for one of their researchers because they 
> were so
> insistent to have two different solutions. Are they the same?
> 
> Well, today I have a request to put tissue for a researcher in 
> formalinand paraformaldehyde. So.... Without percentage 
> required, do I use 10%
> NBF? Do I call somewhere and get paraformaldehyde and make 4%
> paraformaldehyde?
> 
> I have asked the surgeon twice for the number for the lab so I 
> can find
> out - don't have it yet. I have two fresh adrenals in the 
> fridge. Help!!
> 
> 
> Thanks in advance...
> Joyce
> 
> Joyce Weems
> Pathology Manager
> Saint Joseph's Hospital
> 5665 Peachtree Dunwoody Rd NE
> Atlanta, GA 30342
> 678-843-7376 - Phone
> 678-843-7831 - Fax
> 
> 
> 
> -----Original Message-----
> From: histonet-boun...@lists.utsouthwestern.edu
> [mailto:histonet-boun...@lists.utsouthwestern.edu] On Behalf Of Pat
> Flannery
> Sent: Thursday, December 11, 2008 11:59 AM
> To: histonet@lists.utsouthwestern.edu
> Subject: [Histonet] Silly Question?
> 
> Please humor me on this if it's obvious (to everyone but 
> me):  why do we
> use paraformaldehyde (which is so inconvenient to make up) 
> rather than
> buffered formalin or just diluted formaldehyde itself?
> 
> It seems that around here, some folks prefer paraformaldehyde 
> (either 2%
> or 4%) and others use formalin, while some others stick to diluted
> formaldehyde (I see all 4 on labels for specimens submitted for
> histology).  Is it mostly a matter of personal preference 
> or where you
> were trained (i.e. force of habit) or is there a valid reason to use
> each solution (basically the same chemical once in solution, merely
> buffered or not)?  The only answer I've gotten when I've 
> asked is,
> "That's what we always use."
> 
> Thanks.
> 
> -Pat Flannery (not a "real" histologist - I just play one in the lab)
> 
> 
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