Re: Ion fluxes in bacteria?

From: /G=Gerhard/S=Nebe-von-Caron/OU=1890CHPE/O=TMGB.URC/@LANGATE.gb.sprint.com
Date: Mon Sep 11 1995 - 05:08:00 EST

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          The ability to measure ion fluxes in bacteria depends on the 
          pumps they possess. A lot of the bugs will pump out your 
          dyes faster than you want. Staining Listeria for example 
          with Rhodamine, we could modulate the extrusion by sodium 
          chloride. The use of pump inhibitors or EDTA does also 
          interfere with the pumps you want to look at. So first hunt 
          for a suitable organism like Micrococcus luteus (no pump, 
          big cell). It stains beautiful in three colour staining 
          experiments regarding membrane potential and membrane 
          integrity. Otherwise you should use an activated probe like 
          a succinimidyl ester or a chloromethyl conjugate (see 
          Molecular Probes) and stain under pump inhibited conditions. 
          Once they are crosslinked, you can run the cells in normal 
          mode again.
          
          Good Luck
          
          Gerhard
          
          Gerhard Nebe-v.Caron
          Unilever Research, Colworth Laboratory Sharnbrook, 
          Bedfordshire
          GB - MK44 1LQ
          Tel:    +44(0)1234-222066
          FAX:    +44(0)1234-222344
          E.mail: gerhard.nebe-von-caron@urcgb.sprint.com


______________________________ Reply Separator _________________________________
Subject: Ion fluxes in bacteria?
Author:  Geoff.Osborne@anu.edu.au at INTERNET
Date:    06/09/95 18:46


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Hello,
        This may sound like an unusual question but I had a request
yesterday from a user interested in detecting ion fluxes in bacteria. I
don't know of any references regarding this and wondered if someone might be
able to point me to some. I think the basic idea is to insert a sequence of
interest tagged with LacZ and detect it in those cells expressing it by
flow, and also assess the movement of things like calcium or potassium, and
hopefully see some change related to the inserted sequence.
        Any and all suggestion welcome.
Thanks in advance,
Geoff
======================================================================
Geoffrey Osborne                           |  ____  __ o  Ahh!
Flow Cytometry (FACS LAB)                  |  __   `\ <,_
John Curtin School of Medical Research,    |  __  (*)/ (*)
Australian National University,            |  ==============|
CANBERRA, AUSTRALIA.                       |                |--|
Email: Geoff.Osborne@anu.edu.au            |                   |--|...
-----Surfing the Web?: Try http://jcsmr.anu.edu.au/facshome.html------
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