Synthesis of Bivalent Lactosides Based on Terephthalamide, N,N′-Diglucosylterephthalamide, and Glycophane Scaffolds and Assessment of Their Inhibitory Capacity on Medically Relevant Lectins
Autor: | Trinidad Velasco-Torrijos, Paul V. Murphy, Rosaria Leyden, Sébastien G. Gouin, Sabine André, Hans-Joachim Gabius |
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Rok vydání: | 2009 |
Předmět: |
Glycan
Erythrocytes Glycosylation Stereochemistry Galectins Phthalimides enterocyte-like cells Chemical synthesis monomer/dimer equilibrium chemistry.chemical_compound Molecular recognition Agglutination Tests Lectins Amide Cell Adhesion Humans Glycosyl Glycosides mammalian lectins Glycoproteins biology Organic Chemistry crystal-structure tumor-cells molecular mechanics ligand properties Immobilized Proteins chemistry Drug Design endogenous lectins biology.protein Ugi reaction Azide Plant Lectins binding proteins ab-type lectin |
Zdroj: | The Journal of Organic Chemistry. 74:9010-9026 |
ISSN: | 1520-6904 0022-3263 |
Popis: | Glycan recognition by lectins initiates clinically relevant processes such as toxin binding or tumor spread. Thus, the development of potent inhibitors has a medical perspective. Toward this goal, we report the synthesis of both rigid and flexible bivalent lactosides on scaffolds that include secondary and tertiary terephthalamides and N,N'-diglucosyltereplithalmides. Construction of these compounds involved Schmidt-Michel glycosidation, and amide coupling or Ugi reactions of relevant glycosyl amines in key steps. A glycocluster based on a rigid glycophane was also prepared from coupling of a glucuronic acid derivative and p-xylylenediamine with subsequent ring-closing metathesis. Finally, a more flexible bivalent lactoside was produced from lactosyl azide with use of the copper-catalyzed azide-alkyne cycloaddition. Distances between lactose residues were analyzed computationally as were their orientations for the relatively rigid Subset of compounds. Distinct spacing properties were revealed by varying the structure of the scaffold or by varying the location of the lactose residue on the scaffold. To relate these features to bioactivity a plant toxin and human adhesion/growth-regulatory galectins were used as sensors in three types of assay, i.e. measuring agglutination of erythrocytes, binding to glycans of a surface-immobilized glycoprotein, or binding to human cells. Methodologically, the common hemeagglutination assay was found to be considerably less sensitive than both solid-phase and cell assays. The bivalent compounds were less effective at interfering with glycoprotein binding to the plant toxin than to human lectins. Significantly, a constrained compound was identified that displayed selectivity in its inhibitory potency between galectin-3 and its proteolytically processed form. Conversely, compounds with a high degree of flexibility showed notable ability to protect human cells from plant toxin binding. The applied conjugation chemistry thus Is compatible with the long-term aim to produce potent and selective lectin inhibitors. |
Databáze: | OpenAIRE |
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