DRO

Characterization of proADAMTS5 processing by proprotein convertases.

Longpré, Jean-Michel, McCulloch, Daniel R., Koo, Bon-Hun, Alexander, J. Preston, Apte, Suneel S. and Leduc, Richard 2009, Characterization of proADAMTS5 processing by proprotein convertases., International journal of biochemistry and cell biology, vol. 41, no. 5, pp. 1116-1126, doi: 10.1016/j.biocel.2008.10.008.

Attached Files
Name Description MIMEType Size Downloads

Title Characterization of proADAMTS5 processing by proprotein convertases.
Author(s) Longpré, Jean-Michel
McCulloch, Daniel R.
Koo, Bon-Hun
Alexander, J. Preston
Apte, Suneel S.
Leduc, Richard
Journal name International journal of biochemistry and cell biology
Volume number 41
Issue number 5
Start page 1116
End page 1126
Total pages 11
Publisher Elsevier Ltd.
Place of publication Amsterdam, The Netherlands
Publication date 2009-05
ISSN 1357-2725
1878-5875
Keyword(s) ADAMTS
aggrecanase
metalloprotease
furin
activation
arthritis
Summary ADAMTS5 (aggrecanase-2), a key metalloprotease mediating cartilage destruction in arthritis, is synthesized as a zymogen, proADAMTS5. We report a detailed characterization of the propeptide excision mechanism and demonstrate that it is a major regulatory step with unusual characteristics. Using furin-deficient cells and a furin inhibitor, we found that proADAMTS5 was processed by proprotein convertases, specifically furin and PC7, but not PC6B. Mutagenesis of three sites containing basic residues within the ADAMTS5 propeptide (RRR46, RRR69 and RRRRR261) suggested that proADAMTS5 processing occurs after Arg261. That furin processing was essential for ADAMTS5 activity was illustrated using the known ADAMTS5 substrate aggrecan, as well as a new substrate, versican, an important regulatory proteoglycan during mammalian development. When compared to other ADAMTS proteases, proADAMTS5 processing has several distinct features. In contrast to ADAMTS1, whose furin processing products were clearly present intracellularly, cleaved ADAMTS5 propeptide and mature ADAMTS5 were found exclusively in the conditioned medium. Despite attempts to enhance detection of intracellular proADAMTS5 processing, such as by immunoprecipitation of total ADAMTS5, overexpression of furin, and secretion blockade by monensin, neither processed ADAMTS5 propeptide nor the mature enzyme were found intracellularly, which was strongly suggestive of extracellular processing. Extracellular ADAMTS5 processing was further supported by activation of proADAMTS5 added exogenously to HEK293 cells stably expressing furin. Unlike proADAMTS9, which is processed by furin at the cell-surface, to which it is bound, ADAMTS5 does not bind the cell-surface. Thus, the propeptide processing mechanism of ADAMTS5 has several points of distinction from those of other ADAMTS proteases, which may have considerable significance in the context of osteoarthritis.
Language eng
DOI 10.1016/j.biocel.2008.10.008
Field of Research 060107 Enzymes
060199 Biochemistry and Cell Biology not elsewhere classified
HERDC Research category C1.1 Refereed article in a scholarly journal
HERDC collection year 2009
Copyright notice ©2008, Elsevier Ltd
Persistent URL http://hdl.handle.net/10536/DRO/DU:30018578

Document type: Journal Article
Collections: Faculty of Health
School of Medicine
Connect to link resolver
 
Unless expressly stated otherwise, the copyright for items in DRO is owned by the author, with all rights reserved.

Versions
Version Filter Type
Citation counts: TR Web of Science Citation Count  Cited 79 times in TR Web of Science
Scopus Citation Count Cited 87 times in Scopus Google Scholar Search Google Scholar
Access Statistics: 541 Abstract Views, 1 File Downloads  -  Detailed Statistics
Created: Tue, 08 Sep 2009, 17:03:38 EST by Daniel McCulloch

Every reasonable effort has been made to ensure that permission has been obtained for items included in DRO. If you believe that your rights have been infringed by this repository, please contact drosupport@deakin.edu.au.