Molecular and functional characterization of a glycosylated Galactose-Binding lectin from Mytilus californianus

Efrén García-Maldonado; Patricia Cano-Sánchez; Alejandra Hernández-Santoyo

doi:10.1016/j.fsi.2017.05.057

Molecular and functional characterization of a glycosylated Galactose-Binding lectin from Mytilus californianus

Fish Shellfish Immunol. 2017 Jul:66:564-574. doi: 10.1016/j.fsi.2017.05.057. Epub 2017 May 22.

Authors

Efrén García-Maldonado¹, Patricia Cano-Sánchez¹, Alejandra Hernández-Santoyo²

Affiliations

¹ Departamento de Química de Biomacromoléculas, Instituto de Química, Universidad Nacional Autónoma de México. Circuito Exterior, Ciudad Universitaria, Coyoacán, Cd. Mx. C.P. 04510, Mexico.
² Departamento de Química de Biomacromoléculas, Instituto de Química, Universidad Nacional Autónoma de México. Circuito Exterior, Ciudad Universitaria, Coyoacán, Cd. Mx. C.P. 04510, Mexico. Electronic address: hersan@unam.mx.

PMID: 28546025
DOI: 10.1016/j.fsi.2017.05.057

Abstract

Lectins play crucial roles for innate immune responses in invertebrates by recognizing and eliminating pathogens. In this study, a lectin from the mussel Mytilus californianus (MCL) was identified and characterized. The lectin was purified by affinity chromatography in α-lactose-agarose resin showing an experimental molecular mass of 18000 Da as determined by SDS-PAGE and MALDI-TOF mass spectrometry. It was specific for binding d-galactose and N-Acetyl-d-galactosamine that contained carbohydrate moieties that were also inhibited by melibiose and raffinose. It had the ability to agglutinate all types of human erythrocytes, as well as rabbit red blood cells. Circular dichroism analyzes have indicated that this lectin possessed an α/β fold with a predominance of β structures. This was consistent with the structure of the protein that was determined by the X-ray diffraction techniques. MCL was crystallized in the space group C2₁ and it diffracted to 1.79 Å resolution. Two monomers were found in the asymmetric unit and they formed dimers in solution. The protein has shown to be a member of the β-trefoil family, with three sugar binding sites per monomer. In accord with fluorescence-based thermal shift assays, we observed that the MCL T_m increased about 10 °C in the presence of galactose. Furthermore, we have determined the complete amino acid sequence by cDNA sequencing. The gene had two ORF2 proteins, one resulting in a 180 residue protein with a theoretical molecular mass of 20227 Da, and another resulting in a 150 residue protein with a theoretical molecular mass of 16911 Da. The difference between the theoretical and experimental values was due to the presence of a glycosylation that was observed by the glycosylation assay. A positive microbial agglutination and a growth inhibition activity were observed against Gram-negative and Gram-positive bacteria. The M. californianus lectin is the fourth member of the recently proposed new family of lectins that have been reported to date, occurring only in mollusks belonging to the family Mytilidae. It is the first member to be glycosylated and with a strong tendency to form large oligomers.

Keywords: 3D structure; Antimicrobial activity; Carbohydrate-binding protein; GalNAc/Gal-specific lectin; Glycosylated lectin; Immune system; Innate immunity; Marine mollusks; Mytilus californianus.

MeSH terms

Amino Acid Sequence
Animals
Base Sequence
Escherichia coli / physiology
Galectins / chemistry
Galectins / genetics*
Galectins / immunology*
Lactobacillus plantarum / physiology
Mytilus / classification
Mytilus / genetics*
Mytilus / immunology*
Mytilus / microbiology
Phylogeny

Substances

Galectins