Strains of enterotoxigenic Bacteroides fragilis (ETBF) are associated
with diarrhea in young farm animals and, at least in particular settin
gs, in children, Enterotoxin production by ETBF is currently detected
by a tissue culture assay with HT-29 cells. We hare developed a PCR as
say based ore the detection of the enterotoxin gene to identify ETBF i
n culture and in stool samples, Overall, 113 bacterial strains were ex
amined, including 3 B. fragilis reference strains, 75 B. fragilis isol
ates (comprising 40 ETBF isolates), 20 Bacteroides spp. other than B.
fragilis, and 15 strains belonging to other genera, Complete agreement
was found between the results of the tissue culture assay and those a
f the PCR For our strains, PCR was also used Bu detect ETBF directly i
n fecal samples. Stools from two healthy volunteers were spiked with k
nown numbers of ETBF and were processed by three different methods. A
culture method, which required inoculation of the stools on selective
plates and the collection of the whole bacterial growth (''sweeps''),
was Found to be the most sensitive, PCR performed with the plate sweep
s yielded amplification products with a detection limit of 10(5) to 10
(4) CFU/g of feces. Bg this method 18 samples of diarrheic stools (10
positive and 8 negative for ETBF) mere examined, The results of the PC
R were In accordance with the culture results in all cases, The propos
ed PCR assay represents a diagnostic fool for the rapid identification
of ETBF in culture as well as in fecal samples.