Processing enzyme glucosidase II: proposed catalytic residues and developmental regulation during the ontogeny of the mouse mammary gland

doi:10.1093/glycob/cwh110

Glycobiology Advance Access originally published online on June 9, 2004
Glycobiology 2004 14(10):909-921; doi:10.1093/glycob/cwh110

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Processing enzyme glucosidase II: proposed catalytic residues and developmental regulation during the ontogeny of the mouse mammary gland

Jie Feng², Andrew V. Romaniouk², Siba K. Samal³ and Inder K. Vijay¹^,2

² Department of Animal and Avian Sciences, University of Maryland, College Park MD 20742; ³ Virginia-Maryland Regional College of Veterinary Medicine, University of Maryland, College Park MD 20742

Received on April 2, 2004; revised on June 3, 2004; accepted on June 4, 2004

Following the action of glucosidase I to clip the terminal ${alpha}$ 1,2-linkedglucose, glucosidase II sequentially cleaves the two inner ${alpha}$ 1,3-linkedglucose residues from the Glc ${alpha}$ 1,2Glc ${alpha}$ 1,3Glc ${alpha}$ 1,3Man₉GlcNAc₂ oligosaccharideof the incipient glycoprotein as it undergoes folding and maturation.Glucosidase II belongs to family 31 glycosidases. These enzymesact by the acid-base catalytic mechanism. The cDNA of the wild-typeand several mutant forms of the fusion protein of the enzymein which mutations were introduced in the conserved motif D₅₆₄MNE₅₆₇were expressed in Sf9 cells, and the proteins were purifiedon Ni-NTA matrix. The catalytic activity of the purified proteinswas determined with radioactive Glc₂Man₉GlcNAc₂ substrate. Theresults show that the aspartate and glutamate within the D₅₆₄MNE₅₆₇motif can serve for catalysis, most likely as the acid-basepair within the active site of the enzyme. The developmentalregulation of glucosidase II was studied during the ontogenyof the mouse mammary gland for its growth and differentiation.The mRNA of both ${alpha}$ and ß subunits of the enzyme, immunoreactive ${alpha}$ and ß subunits, and enzyme activity were measuredover the complete developmental cycle. The changes in all theparameters were consistent with similar fluctuations with severalother enzymes of the N-glycosylation machinery reported earlier,reaching a three- to fourfold increase over the basal levelin the virgin gland at the peak of lactation. Altogether itappears that there is a coordinated regulation of the enzymesinvolved in protein N-glycosylation during the development ofthe mouse mammary gland.

¹ To whom correspondence should be addressed; e-mail: ivijay{at}umd.edu

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