Accéder au contenu
MilliporeSigma

A mechanism-based ICAT strategy for comparing relative expression and activity levels of glycosidases in biological systems.

Journal of proteome research (2008-06-20)
Omid Hekmat, Shouming He, R Antony J Warren, Stephen G Withers
RÉSUMÉ

An activity-based isotope-coded affinity tagging (AB-ICAT) strategy for proteome-wide quantitation of active retaining endoglycosidases has been developed. Two pairs of biotinylated, cleavable, AB-ICAT reagents (light H(8) and heavy D(8)) have been synthesized, one incorporating a recognition element for cellulases and the other incorporating a recognition element for xylanases. The accuracy of the AB-ICAT methodology in quantifying relative glycosidase expression/activity levels in any two samples of interest has been verified using several pairs of model enzyme mixtures where one or more enzyme amounts and/or activities were varied. The methodology has been applied to the biomass-degrading secretomes of the soil bacterium, Cellulomonas fimi, under induction by different polyglycan growth substrates to obtain a quantitative profile of the relative expression/activity levels of individual active retaining endoglycanases per C. fimi cell. Such biological profiles are valuable in understanding the strategies employed by biomass-degrading organisms in exploiting environments containing different biomass polysaccharides. This is the first report on the application of an activity-based ICAT method to a biological system.

MATÉRIAUX
Référence du produit
Marque
Description du produit

Sigma-Aldrich
3-[2-N-(Biotinyl)aminoethyldithio]propanoic acid, ≥95%