The production of a discontinuous hemolysis pattern that is characteristic
of hemolysin BL, an enterotoxic and dermonecrotic hemolysin previously desc
ribed, was investigated with 114 Bacillus cereus, two B. thuringiensis and
nine B. mycoides strains. Discontinuous patterns were monitored by a blood
agar gel diffusion assay of 5 h and overnight culture supernatants, and by
direct examination after colony growth on blood agar. For gel diffusion, th
e condition for optimal discontinuous pattern development included the use
of sheep blood agar containing 1-2 mM EDTA, the addition of calf serum (8%
v/v) to supernatants before loading the gels, and incubating at 27 degrees
C; under these conditions the patterns generally appeared within 4 h of inc
ubation. The final percent of strains exhibiting a pattern was 74-78%. For
the colony system, two types of blood agar were used: nutrient agar (NA) an
d brain heart infusion agar with glucose (BHIG) containing 8% calf serum an
d 0.1-1 mM EDTA. Both NA and BHIG, containing 0.1 mM EDTA and incubated at
22 degrees C, gave the highest percent of strains exhibiting a pattern. The
patterns generally appeared between 12 and 28 h. Used in combination, NA a
nd BHIG gave 73-74% of positive B. cereus/thuringiensis. Previous results o
btained with 68 strains (Beecher and Wong, 1994a,b) were confirmed; the gel
diffusion system was improved regarding homogeneity of time range of devel
opment, clarity, stability and final yield of patterns; the conditions for
the colony growth system were chosen to make monitoring compatible with a l
aboratory working schedule. In both cases central hemolytic zones, that can
hamper the observation of the patterns, were decreased. It did not seem th
at B. cereus, B. thuringiensis and B. mycoides can be differentiated on the
basis of production of hemolysin BL. (C) 2000 Elsevier Science B.V. All ri
ghts reserved.