Author: Lew, Rebecca A.; Warner, Fiona J.; Hanchapola, Iresha; Yarski, Michael A.; Manohar, Jay; Burrell, Louise M.; Smith, A. Ian
Title: Angiotensinâ€converting enzyme 2 catalytic activity in human plasma is masked by an endogenous inhibitor Cord-id: rq94lma3 Document date: 2008_3_19
ID: rq94lma3
Snippet: Angiotensinâ€converting enzyme 2 (ACE2) is thought to act in an opposing manner to its homologue, angiotensinâ€converting enzyme (ACE), by inactivating the vasoconstrictor peptide angiotensin II and generating the vasodilatory fragment, angiotensin(1–7). Both ACE and ACE2 are membraneâ€bound ectoenzymes and may circulate in plasma as a consequence of a proteolytic shedding event. In this study, we show that ACE2 circulates in human plasma, but its activity is suppressed by the presence of a
Document: Angiotensinâ€converting enzyme 2 (ACE2) is thought to act in an opposing manner to its homologue, angiotensinâ€converting enzyme (ACE), by inactivating the vasoconstrictor peptide angiotensin II and generating the vasodilatory fragment, angiotensin(1–7). Both ACE and ACE2 are membraneâ€bound ectoenzymes and may circulate in plasma as a consequence of a proteolytic shedding event. In this study, we show that ACE2 circulates in human plasma, but its activity is suppressed by the presence of an endogenous inhibitor. Partial purification of this inhibitor indicated that the inhibitor is small, hydrophilic and cationic, but not a divalent metal cation. These observations led us to develop a method for removal of the inhibitor, thus allowing detection of plasma ACE2 levels using a sensitive quenched fluorescent substrateâ€based assay. Using this technique, ACE2 activity measured in plasma from healthy volunteers (n= 18) ranged from 1.31 to 8.69 pmol substrate cleaved min(−1) ml(−1) (mean ±s.e.m., 4.44 ± 0.56 pmol min(−1) ml(−1)). Future studies of patients with cardiovascular, renal and liver disease will determine whether plasma ACE2 is elevated in parallel with increased tissue levels observed in these conditions.
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