Synthesis of the osmoprotectant glycine betaine in Bacillus subtilis: Characterization of the gbsAB genes

Autor(en): Boch, J
Kempf, B
Schmid, R
Bremer, E
Stichwörter: ALDEHYDE DEHYDROGENASE; CHOLINE-OXIDASE; COPY-NUMBER; DEPENDENT TRANSPORT-SYSTEM; ESCHERICHIA-COLI; HIGH-LEVEL; HIGHER-PLANTS; Microbiology; NUCLEOTIDE-SEQUENCE; OSMOTIC-STRESS; RNA-POLYMERASE
Erscheinungsdatum: 1996
Herausgeber: AMER SOC MICROBIOLOGY
Journal: JOURNAL OF BACTERIOLOGY
Volumen: 178
Ausgabe: 17
Startseite: 5121
Seitenende: 5129
Zusammenfassung: 
Synthesis of the osmoprotectant glycine betaine from the exogenously provided precursor choline or glycine betaine aldehyde confers considerable osmotic stress tolerance to Bacillus subtilis in high-osmolarity media. Using an Escherichia coli mutant (betBA) defective in the glycine betaine synthesis enzymes, we cloned by functional complementation the genes that are required for the synthesis of the osmoprotectant glycine betaine in B. subtilis. The DNA sequence of a 4.1-kb segment from the cloned chromosomal B. subtilis DNA was established, and two genes (gbsA and gbsB) whose products were essential for glycine betaine biosynthesis and osmoprotection were identified. The gbsA and gbsB genes are transcribed in the same direction, are separated by a short intergenic region, and are likely to form an operon. The deduced gbsA gene product exhibits strong sequence identity with members of a superfamily of specialized and nonspecialized aldehyde dehydrogenases. This superfamily comprises glycine betaine aldehyde dehydrogenases from bacteria and plants with known involvement in the cellular adaptation to high-osmolarity stress and drought. The deduced gbsB gene product shows significant similarity to the family of type III alcohol dehydrogenases. B. subtilis mutants with defects in the chromosomal gbsAB genes were constructed by marker replacement, and the growth properties of these mutant strains in high-osmolarity medium were analyzed. Deletion of the gbsAB genes destroyed the choline-glycine betaine synthesis pathway and abolished the ability of B. subtilis to deal effectively with high-osmolarity stress in choline- or glycine betaine aldehyde-containing medium. Uptake of radiolabelled choline was unaltered in the gbsAB mutant strain. The continued intracellular accumulation of choline or glycine betaine aldehyde in a strain lacking the glycine betaine-biosynthetic enzymes strongly interfered with the growth of B. subtilis, even in medium of moderate osmolarity. A single transcription initiation site for gbsAB was detected by high-resolution primer extension analysis. gbsAB transcription was initiated from a promoter with close homology to sigma(A)-dependent promoters and was stimulated by the presence of choline in the growth medium.
ISSN: 00219193
DOI: 10.1128/jb.178.17.5121-5129.1996

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