Structural Analysis of Succinoglycan Oligosaccharides from Sinorhizobium meliloti Strains with Different Host Compatibility Phenotypes

Author:

Simsek Senay1,Wood Karl2,Reuhs Bradley L.3

Affiliation:

1. North Dakota State University, Department of Plant Sciences, Fargo, North Dakota, USA

2. Campus-wide Mass Spectrometry Center, Department of Chemistry, Purdue University, West Lafayette, Indiana, USA

3. Whistler Center for Carbohydrate Research, Department of Food Science, Purdue University, West Lafayette, Indiana, USA

Abstract

ABSTRACT Sinorhizobium meliloti NRG247 has a Fix + phenotype on Medicago truncatula A20 and is Fix on M. truncatula A17, and the phenotype is reversed with S. meliloti NRG185. As the succinoglycan was shown to impact host specificity, an analysis of the succinoglycan oligosaccharides produced by each strain was conducted. The symbiotically active s uccinoglycan t rimeric o ligosaccharides (STOs) from the two S. meliloti strains were compared by chromatography and mass spectrometry, and the analysis of the S. meliloti NRG247 oligosaccharides showed that this strain produces an abundance of STO trimer 1 (T1), containing no succinate (i.e., three nonsuccinylated repeats), yet the low-molecular-weight pool contained no nonsuccinylated monomers (potential repeats). This showed that STO T1 is likely to be the active signal on M. truncatula A20 and that the biosynthesis of the STOs is not a random polymerization of the monomer population. The results also suggest that the fully succinylated STO T7 is required for the infection of M. truncatula A17.

Publisher

American Society for Microbiology

Subject

Molecular Biology,Microbiology

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4. KijneJW. 1992. The rhizobium infection process, p 349–398. In StaceyG BurrisRH EvansHJ (ed), Biological nitrogen fixation. Chapman & Hall, New York, NY.

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