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Publication Date:
January 2007
ISSN:
1437-4315
DOI:
10.1515/BC.2007.026

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Biological Chemistry

Editor-in-Chief: Brüne, Bernhard

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The His-Pro-Phe motif of angiotensinogen is a crucial determinant of the substrate specificity of renin

Tsutomu Nakagawa1 / Jyunji Akaki2 / Ryousuke Satou3 / Masatoshi Takaya4 / Hideyuki Iwata5 / Akemi Katsurada6 / Kazuhiro Nishiuchi7 / Yoshihiro Ohmura8 / Fumiaki Suzuki9 / Yukio Nakamura10

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Citation Information: Biological Chemistry. Volume 388, Issue 2, Pages 237–246, ISSN (Online) 1437-4315, ISSN (Print) 1431-6730, DOI: 10.1515/BC.2007.026, January 2007

Publication History:
Received:
May 31, 2006
Accepted:
August 24, 2006
Published Online:
2007-01-29

Abstract

The amino acid sequence His-Pro-Phe as N-terminal residues 6–8 of the natural renin substrate, angiotensinogen, is conserved among species. We investigated whether this His-Pro-Phe motif functions as the determinant of the substrate specificity of renin. Mutant angiotensinogens in which the Ile-His-Pro-Phe-His-Leu sequence at positions 5–10 of wild-type angiotensinogen was replaced by either His-Pro-Phe-His-Leu-Leu or Ala-Ile-His-Pro-Phe-His were cleaved by renin at the C-terminal side of residues 9 and 11, respectively, while wild-type angiotensinogen was cleaved at residue 10. A triple Ala substitution for the His-Pro-Phe motif of angiotensinogen prevented its cleavage by renin. In contrast, triple Ala substitution for residues 9–11, including the natural site of cleavage by renin, allowed cleavage between the two Ala residues at positions 10 and 11. Furthermore, the 33-residue C-terminal peptide of human megsin, which carries a naturally occurring His-Pro-Phe sequence, was cleaved by renin at the C-terminal side of the His-Pro-Phe-Leu-Phe sequence. These results indicate that the His-Pro-Phe motif of angiotensinogen is a crucial determinant of the substrate specificity of renin. By binding to a corresponding pocket on renin, the His-Pro-Phe motif may act as a molecular anchor to recruit the scissile peptide bond to a favorable site for catalysis.

Keywords: exosite; megsin; molecular anchor; renin-angiotensin system; renin inhibitor; substrate specificity

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