Differentiation of Acinetobacter calcoaceticus sensu stricto from related Acinetobacter species by electrophoretic polymorphism of malate dehydrogenase, glutamate dehydrogenase and catalase.

Acinetobacter baumannii, unnamed Acinetobacter species 3 (studied by P.J.M. Bouvet and P.A.D. Grimont) and unnamed DNA group 13 (studied by I. Tjernberg and J. Ursing) are the most prevalent Acinetobacter species in hospitals. Using the identification scheme of Bouvet and Grimont, it is sometimes difficult to differentiate these species from A. calcoaceticus sensu stricto, a species of the natural environment that has seldom been found associated with human infection. Genetically identified Acinetobacter isolates belonging to A. calcoaceticus sensu stricto (n = 12), A. baumannii (n = 22), Acinetobacter species 3 (n = 15) and DNA group 13 of Tjernberg and Ursing (n = 26), Acinetobacter species 10 (n = 2), Acinetobacter species 11 (n = 2) and 3 strains ungrouped by DNA-DNA hybridization were investigated for electrophoretic separations of L-malate dehydrogenase (MDH), glutamate dehydrogenase (GDH) and catalase (CAT). All A. calcoaceticus sensu stricto isolates were easily differentiated from those of other species investigated by their high MDH values (relative mobility (Rf) = 78), their low GDH values (Rf range: 24-28) and CAT values (Rf range: 34-42). Acinetobacter species 3 was differentiated from A. baumannii and DNA group 13 of Tjernberg and Ursing by high CAT values. A. baumannii could not be differentiated from Tjernberg and Ursing DNA group 13. Acinetobacter species 10 was clearly differentiated from Acinetobacter species 11. Once an Acinetobacter is phenotypically identified with the four closely related species investigated here, electrophoretic analysis of MDH, GDH and CAT might be a useful complement to the identification scheme of Bouvet and Grimont for accurately identifying A. calcoaceticus sensu stricto.

Evaluation of two colored latex kits, the Wellcolex Colour Salmonella Test and the Wellcolex Colour Shigella Test, for serological grouping of Salmonella and Shigella species.

Two colored latex kits (the Wellcolex Colour Salmonella Test [WCT-Salmonella] and the Wellcolex Colour Shigella Test [WCT-Shigella]; Division Diagnostics, Laboratories Wellcome S.A., Paris, France), which allow identification of the most frequently encountered Salmonella serogroups and Shigella species, respectively, were evaluated. WCT-Salmonella and WCT-Shigella yielded sensitivities of 98.4 and 98%, respectively, and a specificity of 100% when they were tested on pure cultures received at a reference laboratory.

Species, biotype, and bacteriophage type determinations compared with cell envelope protein profiles for typing Acinetobacter strains.

Species, biotypes, and phage types were determined for 120 Acinetobacter strains from clinical or environmental sources or from culture collections. These characteristics were compared with cell envelope protein profiles obtained by sodium dodecyl sulfate-polyacrylamide gel electrophoresis in previous studies. A considerable heterogeneity of species and types was observed by use of the various methods, in particular among strains from different sources. Acinetobacter baumannii was the most commonly found species in isolates from clinical sources, followed by Acinetobacter species 3. Nine biotypes were observed among A. baumannii strains. Further differentiation within most species and biotypes was achieved by protein profile typing and, to some extent, phage typing. Of 120 strains, 49 (41%) were not typeable by phages. Consistent results for the various classification methods were obtained for strains from common sources. Biotyping seemed an appropriate method for the screening of strains, whereas protein profile and phage typing could serve as additional methods to establish the identity or nonidentity of strains. Results of this study suggest that the combination of the typing methods is useful in epidemiological studies.

Delineation of new proteolytic genomic species in the genus Acinetobacter.

Twenty-seven proteolytic Acinetobacter strains differing phenotypically from the 12 previously described Acinetobacter species were studied by DNA/DNA hybridization using the S1 nuclease method to assess their relatedness. Five DNA groups (genomic species 13 to 17) containing 20 strains were delineated. Seven strains remained ungrouped. Within species, the level of DNA relatedness to the reference strains ranged from 64 to 99%, with delta Tm values below 3.5 degrees C. DNA group 13 was 31 to 42% related to group 14. DNA group 15 was 59 to 69% related to group 16, with delta Tm values between 4.5 and 6 degrees C. DNA group 17 was 51 to 61% related to DNA groups 15 and 16 with delta Tm values between 5.5 and 7.5 degrees C. The seven ungrouped strains were 28 to 60% related to the five newly delineated genomic species with delta Tm between 6.5 and 13.5 degrees C. Reference strains of the five genomic species were 5 to 22% related to the type or reference strains of the 12 Acinetobacter genomic species previously described. Biochemically, DNA groups 13 to 17 and ungrouped strains could not be separated unambiguously and therefore are not named.

[Possible action of riboflavin (vitamin B2) as a chemical telemediator in aquatic ecosystems (author's transl)]. / Intervention possible de la riboflavine (vitamine B2) comme télémédiateur chimique dans les écosystèmes aquatiques.

The attractive action of riboflavin at certain concentrations on the young Salmon (parr) has been demonstrated. This property diminished or disappears with smoltifications. Owing to the emission of riboflavin by the young Salmon, the possibility, at diverse migratory or sedentary phases of the biological cycle, of an action of a pheromone or ecomone type, is discussed.