Renal metabolism of calcitonin
- 1 April 1988
- journal article
- research article
- Published by American Physiological Society in American Journal of Physiology-Renal Physiology
- Vol. 254 (4) , F593-F600
- https://doi.org/10.1152/ajprenal.1988.254.4.f593
Abstract
The kidneys account for approximately two-thirds of the metabolism of calcitonin, but relatively little is known regarding the details thereof. To further characterize this process, we examined the renal handling and metabolism of human calcitonin (hCT) by the isolated perfused rat kidney. We also studied the degradation of radiolabeled salmon calcitonin (sCT) by subcellular fractions prepared from isolated rabbit proximal tubules. The total renal (organ) clearance of immunoreactive hCT by the isolated kidney was 1.96 .+-. 0.18 ml/min. This was independent of the perfusate total calcium concentration from 5.5 to 10.2 mg/dl. Total renal clearance exceeded the glomerular filtration rate (GFR, 0.68 .+-. 0.05 ml/min), indicating filtration-independent removal. Urinary calcitonin clearance as a fraction of GFR averaged 2.6%. Gel filtration chromatography of medium from isolated kidneys perfused with 125I-labeled sCT showed the principal degradation products to be low molecular weight forms eluting with monoiodotyrosine. Intermediate size products were not detected. In the subcellular fractionation experiments, when carried out at pH 5.0, calcitonin hydrolysis exclusively followed the activities of the lysosomal enzyme N-acetyl-.beta.-glucosaminidase. Typically, at pH 7.5, 42% of total degradation occurred in the region of the brush-border enzyme alanyl aminopeptidase and 29% occurred in the region of the cytosolic enzyme phosphoglucomutase. Although 9% of the calcitonin-degrading activity was associated with basolateral membrane fractions, most of this activity could be accounted for by the presence of brush-border membranes. We conclude that renal removal of calcitonin proceeds through filtration and filtration-independent pathways and that hydrolysis of filtered calcitonin likely occurs at the level of the brush-border membranes. Because proximal tubule basolateral membrane fractions exhibit low degrading activity and filtration-independent removal is large, this raises the question whether calcitonin is degraded at nonproximal tubular sites or by other mechanisms such as endocytosis at the basolateral membranes and delivery to lysosomes.This publication has 15 references indexed in Scilit:
- Effect of estrogens and phosphorus depletion on plasma calcitonin in the ratCalcified Tissue International, 1983
- Fate of [125I]insulin removed from the peritubular circulation of isolated perfused rat kidneyAmerican Journal of Physiology-Renal Physiology, 1982
- Differences between renal tubular processing of glucagon and insulinAmerican Journal of Physiology-Renal Physiology, 1982
- Analytical cell fractionation of isolated rabbit renal proximal tubulesKidney International, 1981
- Removal and excretion of immunoreactive rat growth hormone by the isolated kidneyAmerican Journal of Physiology-Renal Physiology, 1981
- Direct in vivo demonstration by radioautography of specific binding sites for calcitonin in skeletal and renal tissues of the rat.The Journal of cell biology, 1980
- The Handling of Immunoreactive Vasopressin by the Isolated Perfused Rat KidneyJournal of Clinical Investigation, 1979
- Plasma kinetics and urinary excretion of exogenous human and salmon calcitonin in man.American Journal of Physiology-Endocrinology and Metabolism, 1979
- Factors Influencing the Handling of Insulin by the Isolated Rat KidneyJournal of Clinical Investigation, 1978
- Degradation of parathyroid hormone and fragment production by the isolated perfused dog kidney. The effect of glomerular filtration rate and perfusate CA++ concentrations.Journal of Clinical Investigation, 1977