Affiliation:
1. Department of Food Science, Cornell University, Ithaca, New York 14853
Abstract
ABSTRACT
Genetic and biochemical evidence for a defective xylan degradation pathway was found linked to the xylose operon in three lactococcal strains,
Lactococcus lactis
210,
L. lactis
IO-1, and
L. lactis
NRRL B-4449. Immediately downstream of the xylulose kinase gene (
xylB
) (K. A. Erlandson, J.-H. Park, W. El Khal, H.-H. Kao, P. Basaran, S. Brydges, and C. A. Batt, Appl. Environ. Microbiol. 66:3974–3980, 1999) are two open reading frames encoding a mutarotase (
xylM
) and a xyloside transporter (
xynT
) and a partial open reading frame encoding a β-xylosidase (
xynB
). These are functions previously unreported for lactococci or lactobacilli. The mutarotase activity of the putative
xylM
gene product was confirmed by overexpression of the
L. lactis
enzyme in
Escherichia coli
and purification of recombinant XylM. We hypothesize that the mutarotase links xylan degradation to xylose metabolism due to the anomeric preference of xylose isomerase. In addition, Northern hybridization experiments suggested that the
xylM
and
xynTB
genes are cotranscribed with the
xylRAB
genes, responsible for xylose metabolism. Although none of the three strains appeared to metabolize xylan or xylobiose, they exhibited xylosidase activity, and
L. lactis
IO-1 and
L. lactis
NRRL B-4449 had functional mutarotases.
Publisher
American Society for Microbiology
Subject
Ecology,Applied Microbiology and Biotechnology,Food Science,Biotechnology
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