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Appl. Environ. Microbiol., Apr 1997, 1564-1569, Vol 63, No. 4
S Saby, I Sibille, L Mathieu, JL Paquin and JC Block
Counting bacteria in drinking water samples by the epifluorescence
technique after 4',6-diamidino-2-phenylindole (DAPI) staining is
complicated by the fact that bacterial fluorescence varies with exposure of
the cells to sodium hypochlorite. An Escherichia coli laboratory-grown
suspension treated with sodium hypochlorite (5 to 15 mg of chlorine
liter-1) for 90 min was highly fluorescent after DAPI staining probably due
to cell membrane permeation and better and DAPI diffusion. At chlorine
concentrations greater than 25 mg liter-1, DAPI- stained bacteria had only
a low fluorescence. Stronger chlorine doses altered the DNA structure,
preventing the DAPI from complexing with the DNA. When calf thymus DNA was
exposed to sodium hypochlorite (from 15 to 50 mg of chlorine liter-1 for 90
min), the DNA lost the ability to complex with DAPI. Exposure to
monochloramine did not have a similar effect. Treatment of drinking water
with sodium hypochlorite (about 0.5 mg of chlorine liter-1) caused a
significant increase in the percentage of poorly fluorescent bacteria, from
5% in unchlorinated waters (40 samples), to 35 to 39% in chlorinated waters
(40 samples). The presence of the poorly fluorescent bacteria could explain
the underestimation of the real number of bacteria after DAPI staining.
Microscopic counting of both poorly and highly fluorescent bacteria is
essential under these conditions to obtain the total number of bacteria. A
similar effect of chlorination on acridine orange-stained bacteria was
observed in treated drinking waters. The presence of the poorly fluorescent
bacteria after DAPI staining could be interpreted as a sign of dead cells.
Copyright © 1997, American Society for Microbiology
Influence of water chlorination on the counting of bacteria with DAPI (4',6-diamidino-2-phenylindole)
GIP Stelor/Laboratoire d'Hygiene et de Recherche en Sante Publique, Vandoeuvre les Nancy, France.
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