In vitro expression of a 22-kilodalton Yersinia pestis polypeptide immunologically related to the 25-kilodalton plasmid-encoded protein of the three pathogenic Yersinia species.

Antibodies raised against the 25-kilodalton (p25) plasmid-encoded polypeptide of Yersinia enterocolitica recognized the homologous protein in the three Yersinia species grown in vitro. This polypeptide was recovered from whole cells as well as from the fluid supernatant of bacteria grown at 37 degrees C in a Ca2+-deficient medium. Furthermore, a 22-kilodalton (p22) plasmid-encoded polypeptide immunologically related to p25 was found only in Y.

Ability of Yersinia enterocolitica cells to inactivate bacteriophage I at 25 degrees and 37 degrees C.

The presence of receptors to bacteriophage I of Y. enterocolitica in Y. enterocolitica cells grown at 37 degrees C was investigated.

Lack of correlation between plasmid-encoded outer membrane proteins and virulence of Yersinia enterocolitica.

When various strains of Yersinia enterocolitica belonging to serovars 0:1,3, 0:3, 0:5,27, 0:9 and 0:Tacoma harbouring 44- to 47-Md plasmids, or their spontaneously cured isogenic pairs, were inoculated (i. v., with standardized inocula) into Swiss female mice, the kinetics of bacterial survival in the spleen were followed, revealing inoculum destruction within 15 days.

Pigmented strains of Yersinia intermedia isolated from water.

Two Yersinia intermedia strains isolated from water produced a nondiffusible blue-grey pigment. Pigment production was influenced by culture conditions: it was inhibited at 37 degrees C and by growth in anaerobiosis. Dissociation into non-pigmented clones occurred spontaneously.

Temperature-modulated immunogenicity to Yersinia pestis from Yersinia enterocolitica O3.

The ability of Yersinia enterocolitica O3, grown at 25 degrees C, to promote cross-immunity to Y. pestis was lost after repeated subcultures at 37 degrees C, which selected for bacterial populations having lower in vivo survival. Subculturing Y.