Your search keyword '"Klarskov, Letty"' showing total 4 results

1. Neutral endopeptidase 24.11 is important for the degradation of both endogenous and exogenous glucagon in anesthetized pigs

Author

Trebbien, Ramona, Klarskov, Letty, Olesen, Mette, Holst, Jens J., Carr, Richard D., and Deacon, Carolyn F.

Subjects

Swine -- Physiological aspects, Enzyme inhibitors, Glucagon, Biological sciences

Abstract

Glucagon has a short plasma [t.sub.1/2] in vivo, with renal extraction playing a major role in its elimination. Glucagon is degraded by neutral endopeptidase (NEP) 24.11 in vitro, but the physiological relevance of NEP 24.11 in glucagon metabolism is unknown. Therefore, the influence of candoxatril, a selective NEP inhibitor, on plasma levels of endogenous and exogenous glucagon was examined in anesthetized pigs. Candoxatril increased endogenous glucagon concentrations, from 6.3 [+ or -] 2.5 to 20.7 [+ or -] 6.3 pmol/l [COOH-terminal (C)-RIA, P < 0.05]. During glucagon infusion, candoxatril increased the [t.sub.1/2] determined by C-RIA (from 3.0 [+ or -] 0.5 to 17.0 [+ or -] 2.5 min, P < 0.005) and midregion (M)-RIA (2.8 [+ or -] 0.5 to 17.0 [+ or -] 3.0 min, P < 0.01) and reduced metabolic clearance rates (MCR; 19.1 [+ or -] 3.2 to 9.4 [+ or -] 2.0 ml*[kg.sup.-1]*[min.sup.-1], P < 0.02, C-RIA; 19.2 [+ or -] 4.8 to 9.0 [+ or -] 2.3 ml*[kg.sup.-1]*[min.sup.-1], P < 0.05, M-RIA). However, neither [t.sub.1/2] nor MCR determined by N[H.sub.2]-terminal (N)-RIA were significantly affected ([t.sub.1/2], 2.7 [+ or -] 0.4 to 4.5 [+ or -] 1.6 min; MCR, 30.3 [+ or -] 6.4 to 28.5 [+ or -] 9.0 ml*[kg.sup.-1]*[min.sup.-1]), suggesting that candoxatril had no effect on N[H.sub.2]-terminal degradation but leads to the accumulation of N[H.sub.2]-terminally truncated forms of glucagon. Determination of arteriovenous glucagon concentration differences revealed that renal glucagon extraction was reduced (but not eliminated) by candoxatril (from 40.4 [+ or -] 3.8 to 18.6 [+ or -] 4.1%, P < 0.02, C-RIA; 29.2 [+ or -] 3.1 to 14.7 [+ or -] 2.2%, P < 0.02, M-RIA; 26.5 [+ or -] 4.0 to 19.7 [+ or -] 3.5%, P < 0.06, N-RIA). Femoral extraction was reduced by candoxatril when determined by C-RIA (from 22.7 [+ or -] 2.4 to 8.0 [+ or -] 5.1%, P < 0.05) but was not changed significantly when determined using M- or N-RIAs (10.0 [+ or -] 2.8 to 4.7 [+ or -] 3.7%, M-RIA; 10.5 [+ or -] 2.5 to 7.8 [+ or -] 4.2%, N-RIA). This study provides evidence that NEP 24.11 is an important mediator of the degradation of both endogenous and exogenous glucagon in vivo. candoxatril; peptide; enzyme inhibition

Published

2004

2. Differential regional metabolism of glucagon in anesthetized pigs

Author

Deacon, Carolyn F., Kelstrup, Mette, Trebbien, Ramona, Klarskov, Letty, Olesen, Mette, and Holst, Jens J.

Subjects

Proteases -- Research, Metabolism -- Research, Biological sciences

Abstract

Glucagon metabolism under basal (endogenous) conditions and during intravenous glucagon infusion was studied in anesthetized pigs by use of midregion (M), COOH-terminal (C), and N[H.sub.2]-terminal (N)-RIAs. Arteriovenous concentration differences revealed a negative extraction of endogenous glucagon immunoreactivity across the portal bed (-35.4 [+ or -] 11.0, -40.3 [+ or -] 9.6, -35.6 [+ or -] 16.9%, M-, C-, N-RIA, respectively), reflecting net secretion of pancreatic glucagon and intestinal glicentin and oxyntomodulin, but under exogenous conditions, a net extraction occurred (11.6 [+ or -] 3.6 and 18.6 [+ or -] 5.7%, C- and N-RIA, respectively). Hindlimb extraction of endogenous (17.4 + 3.7%, C-RIA) and exogenous (29.1 [+ or -] 4.8 and 19.8 [+ or -] 5.1%, C- and M-RIA) glucagon was detected, indicating M and C cleavage of the molecule. Renal extraction of glucagon was detected by all assays under endogenous (19.4 [+ or -] 6.7, 33.9 [+ or -] 7.1, 29.5 [+ or -] 6.7%, M-, C-, N-RIA) and exogenous conditions (46.9 [+ or -] 4.8, 46.4 [+ or -] 6.0, 47.0 [+ or -] 7.7%; M-, C-, N-RIA), indicating substantial elimination of the peptide. Hepatic glucagon extraction was undetectable under basal conditions and detected only by M-RIA (10.0 [+ or -] 3.8%) during gtucagon infusion, indicating limited midregional cleavage of the molecule. The plasma half-life determined by C- and N-RIAs (2.7 [+ or -] 0.2 and 2.3 [+ or -] 0.2 min) were similar, but both were shorter than when determined by M-RIA (3.2 [+ or -] 0.2 min, P < 0.02). Metabolic clearance rates were similar regardless of assay (14.4 [+ or -] 1.1, 13.6 [+ or -] 1.7, 17.0 [+ or -] 1.7 ml*[kg.sup.-1]*[min.sup.-1], M-, C-, N-RIA). Porcine plasma degraded glucagon, but this was not significantly affected by the dipeptidyl peptidase IV (DPP IV) inhibitor valine-pyrrolidide, and in anesthetized pigs, glucagon's metabolic stability was unchanged by DPP IV inhibition. We conclude that tissue-specific metabolism of glucagon occurs, with the kidney being the main site of removal and the liver playing little, if any, role. Furthermore, valine-pyrrolidide has no effect on glucagon stability, suggesting that DPP IV is unimportant in glucagon metabolism in vivo, in contrast to its significant role in the metabolism of the other proglucagon-derived peptides and glucose-dependent insulinotropic polypeptide. dipeptidyl peptidase IV; valine-pyrrolidide; peptide degradation

Published

2003

3. Dipeptidyl Peptidase IV Inhibition Reduces the Degradation and Clearance of GIP and Potentiates Its Insulinotropic and Antihyperglycemic Effects in Anesthetized Pigs

Author

Deacon, Carolyn F., Danielsen, Patricia, Klarskov, Letty, Olesen, Mette, and Holst, Jens J.

Published

2001

4. Differential regional metabolism of glucagon in anesthetized pigs.

Author

Deacon, Carolyn F, Kelstrup, Mette, Trebbien, Ramona, Klarskov, Letty, Olesen, Mette, Holst, Jens J, Deacon, Carolyn F, Kelstrup, Mette, Trebbien, Ramona, Klarskov, Letty, Olesen, Mette, and Holst, Jens J

Abstract

Udgivelsesdato: 2003-Sep, Glucagon metabolism under basal (endogenous) conditions and during intravenous glucagon infusion was studied in anesthetized pigs by use of midregion (M), COOH-terminal (C), and NH2-terminal (N)-RIAs. Arteriovenous concentration differences revealed a negative extraction of endogenous glucagon immunoreactivity across the portal bed (-35.4 +/- 11.0, -40.3 +/- 9.6, -35.6 +/- 16.9%, M-, C-, N-RIA, respectively), reflecting net secretion of pancreatic glucagon and intestinal glicentin and oxyntomodulin, but under exogenous conditions, a net extraction occurred (11.6 +/- 3.6 and 18.6 +/- 5.7%, C- and N-RIA, respectively). Hindlimb extraction of endogenous (17.4 +/- 3.7%, C-RIA) and exogenous (29.1 +/- 4.8 and 19.8 +/- 5.1%, C- and M-RIA) glucagon was detected, indicating M and C cleavage of the molecule. Renal extraction of glucagon was detected by all assays under endogenous (19.4 +/- 6.7, 33.9 +/- 7.1, 29.5 +/- 6.7%, M-, C-, N-RIA) and exogenous conditions (46.9 +/- 4.8, 46.4 +/- 6.0, 47.0 +/- 7.7%; M-, C-, N-RIA), indicating substantial elimination of the peptide. Hepatic glucagon extraction was undetectable under basal conditions and detected only by M-RIA (10.0 +/- 3.8%) during glucagon infusion, indicating limited midregional cleavage of the molecule. The plasma half-life determined by C- and N-RIAs (2.7 +/- 0.2 and 2.3 +/- 0.2 min) were similar, but both were shorter than when determined by M-RIA (3.2 +/- 0.2 min, P < 0.02). Metabolic clearance rates were similar regardless of assay (14.4 +/- 1.1, 13.6 +/- 1.7, 17.0 +/- 1.7 ml x kg-1 x min-1, M-, C-, N-RIA). Porcine plasma degraded glucagon, but this was not significantly affected by the dipeptidyl peptidase IV (DPP IV) inhibitor valine-pyrrolidide, and in anesthetized pigs, glucagon's metabolic stability was unchanged by DPP IV inhibition. We conclude that tissue-specific metabolism of glucagon occurs, with the kidney being the main site of removal and the liver playing little, if any, role. Furthermore, valin

Published

2003