Lewis A

Lewis A

Lewis A (Lea) is a fucosylated trisaccharide antigen within the histo-blood group carbohydrate family, characterized by the structure Galβ(1→3)[Fucα(1→4)]GlcNAcβ, where galactose (Gal) links β1-3 to N-acetylglucosamine (GlcNAc), and fucose (Fuc) attaches α1-4 to the same GlcNAc residue. This type I chain differs from type II chains like Lewis X by the β1-3 Gal-GlcNAc linkage instead of β1-4. The core monosaccharides—Gal, Fuc, and GlcNAc—contribute to its specificity, with NMR signals aiding structural confirmation, such as H-1 at ~4.70 ppm for GlcNAc and ~4.65 ppm for the terminal Gal.

Biosynthesis and Genetic Basis

Synthesis of Lewis A relies on fucosyltransferases encoded by the FUT3 gene, adding α1-4 Fuc to the type I precursor Galβ1-3GlcNAc, while the secretor FUT2 gene adds α1-2 Fuc to form difucosylated Lewis B. Lea expression predominates in non-secretors (se/se genotype) with active FUT3, appearing in secretions like milk and plasma, and correlating with Lewis blood group phenotyping. Elongation often occurs in Lea-carrying chains, unlike shorter Leb structures.

Biological Roles and Clinical Relevance

Lewis A antigens function in cell adhesion, serving as ligands for selectins during inflammation and contributing to sialyl Lewis A (sLea) in cancer metastasis. Found on glycoproteins and glycolipids in human milk oligosaccharides, they influence microbial interactions and immune responses. In oncology, Ley (a related antigen) marks tumor cells, prompting synthesis efforts for therapeutic targets.

Synthetic Approaches

Automated glycan assembly and orthogonal glycosylation enable efficient Lea production, using fucosyl fluorides and selective deprotection to build the trisaccharide core. These methods yield pure antigens for studies, often extending to longer chains like KH-1 nonasaccharide. Structural elucidation employs MS fragmentation (B/Y ions) and NMR for linkage verification.

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