Affiliation:
1. Laboratory of Basic and Applied Molecular Biotechnology, Graduate School of Agriculture, Kyoto University, Uji, Kyoto 611-0011, Japan
Abstract
ABSTRACT
Plant cell wall degradation is a premier event when
Bacillus subtilis
, a typical saprophytic bacterium, invades plants. Here we show the degradation system of rhamnogalacturonan type I (RG-I), a component of pectin from the plant cell wall, in
B. subtilis
strain 168. Strain 168 cells showed a significant growth on plant cell wall polysaccharides such as pectin, polygalacturonan, and RG-I as a carbon source. DNA microarray analysis indicated that three gene clusters (
yesOPQRSTUVWXYZ
,
ytePQRST
, and
ybcMOPST-ybdABDE
) are inducibly expressed in strain 168 cells grown on RG-I. Cells of an industrially important bacterium,
B. subtilis
strain natto, fermenting soybeans also express the gene cluster including the
yes
series during the assimilation of soybean used as a carbon source. Among proteins encoded in the
yes
cluster, YesW and YesX were found to be novel types of RG lyases releasing disaccharide from RG-I. Genetic and enzymatic properties of YesW and YesX suggest that strain 168 cells secrete YesW, which catalyzes the initial cleavage of the RG-I main chain, and the resultant oligosaccharides are converted to disaccharides through the extracellular exotype YesX reaction. The disaccharide is finally degraded into its constituent monosaccharides through the reaction of intracellular unsaturated galacturonyl hydrolases YesR and YteR. This enzymatic route for RG-I degradation in strain 168 differs significantly from that in plant-pathogenic fungus
Aspergillus aculeatus
. This is, to our knowledge, the first report on the bacterial system for complete RG-I main chain degradation.
Publisher
American Society for Microbiology
Subject
Ecology,Applied Microbiology and Biotechnology,Food Science,Biotechnology
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