Newsgroups: sci.bio
Path: utzoo!utgpu!news-server.csri.toronto.edu!mailrus!sharkey!msuinfo!midway!ux1.cso.uiuc.edu!brutus.cs.uiuc.edu!wuarchive!mit-eddie!bloom-beacon!athena.mit.edu!whycare
From: whycare@athena.mit.edu (nemo)
Message-ID: <1990Jun29.234444.13873@athena.mit.edu>
Sender: news@athena.mit.edu (News system)
Reply-To: whycare@athena.mit.edu (nemo)
Organization: Massachusetts Institute of Technology
Subject:More on DNA Purification 
Date: Fri, 29 Jun 90 23:44:44 GMT
Lines: 44

Having received several e-mail responses to my last posting on DNA
Purification,
I came up with some more questions of interest: 

1) Why does protein and not DNA partition out into the
phenol/chloroform/(isoamyl    alcohol) phase in the organic solvent
extraction? 

2) What phases would I see in a test tube if I took a DNA/some unwanted
protein      sample suspended in 70% ethanol high salt concentration,
added an equal volume    of phenol/chloroform/isoamyl alcohol (24:24:1),
mixed and then centrifuged the    entire mixture? Here's my guess:

   TOP OF TUBE
 
   organic phase (phenol/chloroform/alcohol)
   white interface  (protein)
   aqueous phase  (water)
   DNA pellet
   
   BOTTOM OF TUBE

   Then to get the purified DNA, I'd remove the organic phase and white
interface
   and vacuum-dry the pellet.

   Is the above procedure orthodox?
   If not, what is orthodox?
   What would I really see if I'm wrong about my guess?

************************************************************************
********** 
Send e-mail to: whycare@athena.mit.edu
************************************************************************
**********
Send USnail mail to:|  
Ruth C. Wang        | Life is too long. If I had the courage to end it,
I would.
Senior House        | Too bad I'm a coward.
Nichols 105         |
4 Ames Street       | 
Cambridge, MA 02139 |
************************************************************************
**********
