Colony growth of protozoan parasites in agar can be useful for axenization,
cloning, and viability studies. This is usually achieved with the pour pla
te method, for which the parasite colonies are situated within the agar. Th
is technique has been described for Giardia intestinalis. Trichomonas vagin
alis, and Entamoeba and Blastocystis species. Extracting such colonies can
be laborious. It would be especially useful if parasites could be grown on
agar as colonies. These colonies, being exposed on the agar surface, could
be conveniently isolated for further investigation. In this study, we repor
t the successful culture of B. hominis cells as colonies on solid agar. Col
onies were enumerated and the efficiency of plating was determined. It was
observed that B. hominis could be easily cultured on agar as clones. The co
lonies were dome-shaped and mucoid and could grow to 3 mm in diameter. Flow
cytometric analyses revealed that parasite colonies remained viable for up
to 2 weeks. Viable colonies were conveniently expanded in liquid or solid
media. Scanning electron microscopy revealed that each colony consists of t
wo regions; a dome-shaped, central core region and a flattened, peripheral
region. Older colonies possessed numerous strand-like surface coat projecti
ons. This study provides the first report of clonal growth of B. hominis on
agar and a simple, effective method for cloning and expansion of B. homini
s cells. (C) 2000 Academic Press.