Effect of N-linked glycosylation on the aspartic proteinase porcine pepsin expressed from Pichia pastoris

doi:10.1093/glycob/cwh024

Glycobiology Advance Access originally published online on December 23, 2003

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Glycobiology vol 14 no 5 pp. 417-429, 2004
Glycobiology vol. 14 no. 5 © Oxford University Press 2004; all rights reserved.

Effect of N-linked glycosylation on the aspartic proteinase porcine pepsin expressed from Pichia pastoris

Mark A. Yoshimasu², Takuji Tanaka³, Jong-Kun Ahn⁴ and Rickey Y. Yada¹^,2

² Department of Food Science, University of Guelph, Guelph, Ontario, Canada N1G 2W1; ³ Department of Applied Microbiology and Food Science, University of Saskatchewan, Saskatoon, Saskatchewan, Canada S7N 5A8; ⁴ Department of Agricultural Science, Korea National Open University,169, Dongsung-Dong, Chongro-Ku, Seoul, 110-791, Korea

Received on August 1, 2003; revised on October 16, 2003; accepted on October 21, 2003

A study was undertaken to examine the effects of N-linked glycosylationon the structure-function of porcine pepsin. The N-linked motifwas incorporated into four sites (two on the N-terminal domainand two on the C-terminal domain), and the recombinant proteinexpressed using Pichia pastoris. All four N-linked recombinantsexhibited similar secondary and tertiary structure to nonglycosylatedpepsin, that is, wild type. Similar K_m values were observed,but catalytic efficiencies were approximately one-third forall mutants compared with the wild type; however, substratespecificity was not altered. Activation of pepsinogen to pepsinoccurred between pH 1.0 to 4.0 for wild-type pepsin, whereasthe glycosylated recombinants activated over a wider range,pH 1.0 to 6.0. Glycosylation on the C-terminal domain exhibitedsimilar pH activity profiles to nonglycosylated pepsin, andglycosylation on the N-domain resulted in a change in activityprofile. Overall, glycosylation on the C-domain led to a moreglobal stabilization of the structure, which translated intoenzymatic stability, whereas on the N-domain, an increase instructural stability had little effect on enzymatic stability.Finally, glycosylation on the flexible loop region also appearedto increase the overall structural stability of the proteincompared with wild type. It is postulated that the presenceof the carbohydrate residues added rigidity to the protein structureby reducing conformational mobility of the protein, therebyincreasing the structural stability of the protein.

¹ To whom correspondence should be addressed; e-mail: ryada{at}uoguelph.ca

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