Abstract
ACE chimeric proteins and N domain monoclonal antibodies (mAbs) were used to determine the influence of the N domain, and particular regions thereof, on the rate of ACE ectodomain shedding. Somatic ACE (having both N and C domains) was shed at a rate of 20%/24 h. Deletion of the C domain of somatic ACE generated an N domain construct (ACEΔC) which demonstrated the lowest rate of shedding (12%). However, deletion of the N domain of somatic ACE (ACEAN) dramatically increased shedding (212%). Testicular ACE (tACE) having 36 amino acid residues (heavily O-glycosylated) at the N-terminus of the C domain shows a 4-fold decrease in the rate of shedding (49%) compared to that of ACEΔN. When the N-terminal region of the C domain was replaced with the corresponding homologous 141 amino acids of the N domain (N-delACE) the rate of shedding of the ACEΔN was only slightly decreased (174%), but shedding was still 3.5-fold more efficient than wild-type testicular ACE. Monoclonal antibodies specific for distinct, but overlapping, N-domain epitopes altered the rate of ACE shedding. The mAb 3G8 decreased the rate of shedding by 30%, whereas mAbs 9B9 and 3A5 stimulated ACE shedding 2- to 4-fold. Epitope mapping of these mAbs in conjunction with a homology model of ACE N domain structure, localized a region in the N-domain that may play a role in determining the relatively low rate of shedding of somatic ACE from the cell surface.
Original language | English |
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Pages (from-to) | 258-267 |
Number of pages | 10 |
Journal | Journal of Proteome Research |
Volume | 4 |
Issue number | 2 |
DOIs | |
Publication status | Published - 1 Mar 2005 |
Keywords
- Angiotensin l-converting enzyme
- Epitope mapping
- Monoclonal antibody
- Shedding
ASJC Scopus subject areas
- General Chemistry
- Biochemistry