Back to Search Start Over

Mutations at critical N-glycosylation sites reduce tyrosinase activity by altering folding and quality control.

Authors :
Branza-Nichita N
Negroiu G
Petrescu AJ
Garman EF
Platt FM
Wormald MR
Dwek RA
Petrescu SM
Source :
The Journal of biological chemistry [J Biol Chem] 2000 Mar 17; Vol. 275 (11), pp. 8169-75.
Publication Year :
2000

Abstract

Tyrosinase is a copper-containing enzyme that regulates melanin biosynthesis in mammals. Mutations at a single N-glycosylation sequon of tyrosinase have been reported to be responsible for oculocutaneous albinism type IA in humans, characterized by inactive tyrosinase and the total absence of pigmentation. To probe the role that each N-glycosylation site plays in the synthesis of biologically active tyrosinase, we analyzed the calnexin mediated folding of tyrosinase N-glycosylation mutants. We have determined that four of the six potential N-glycosylation sites, including that associated with albinism, are occupied. Analysis of the folding pathway and activity of 15 tyrosinase mutants lacking one or more of the occupied N-glycosylation sites shows that glycans at any two N-glycosylation sites are sufficient to interact with calnexin and give partial activity, but a specific pair of sites (Asn(86) and Asn(371)) is required for full activity. The mutants with less than two N-glycosylation sites do not interact with calnexin and show a complete absence of enzyme activity. Copper analysis of selected mutants suggests that the observed partial activity is due to two populations with differential copper content. By correlating the degree of folding with the activity of tyrosinase, we propose a local folding mechanism for tyrosinase that can explain the mechanism of inactivation of tyrosinase N-glycosylation mutants found in certain pigmentation disorders.

Details

Language :
English
ISSN :
0021-9258
Volume :
275
Issue :
11
Database :
MEDLINE
Journal :
The Journal of biological chemistry
Publication Type :
Academic Journal
Accession number :
10713140
Full Text :
https://doi.org/10.1074/jbc.275.11.8169