4.4 Article

Urinary oxytocin as a non-invasive biomarker for neurohypophyseal hormone secretion

Journal

PEPTIDES
Volume 27, Issue 11, Pages 2877-2884

Publisher

ELSEVIER SCIENCE INC
DOI: 10.1016/j.peptides.2006.05.007

Keywords

sodium chloride; vasopressin; hypothalamus; genetic models; kidney; osmotic control; mouse

Funding

  1. NHLBI NIH HHS [HL69319] Funding Source: Medline

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The objective was to characterize the urinary oxytocin (OT) system with the goal of using it as a biomarker for neurohypophyseal peptide secretion. We studied urinary OT secretion in mice under three conditions: (1) in OT gene deletion mice (OT-/-) which lack the ability to produce the peptide; (2) after arterial vascular infusion of OT and (3) after physiological stimulation with consumption of 2% sodium chloride. OT was measured by radioimmunoassay (RIA) and Surface-Enhanced Laser Desorption Ionization Time of Flight Mass Spectroscopy (SELDI TOF MS). In OT-/- mice (n = 25), urinary OT levels were not detectable, while in OT+/+ mice (n = 23) levels were 250.2 +/- 35.3 pg/ml. To evaluate blood/urine transfer, mice with chronic carotid arterial catheters were infused with saline or OT (5 or 20 pmol/min). Peak urine OT levels were 89 +/- 11.5 and 844 +/- 181 ng/ml in the low and high OT groups, respectively. Proteomic evaluation showed MS peaks, corresponding to OT (similar to 1009 Da) and a related peptide (1030 Da) with highest levels in mice infused with OT. Salt loading (5 days of 2% NaCl as drinking water) increased plasma osmolality (3.3%), increased plasma and urinary vasopressin (AVP), but caused no changes in OT. Thus, using non-invasive urine samples, we document that urinary OT and AVP can be used to monitor changes in peptide secretion. Urinary OT and AVP, as well as other urinary peptides, may provide a viable biomarker for peptide secretion and may be useful in clinical studies. (c) 2006 Elsevier Inc. All rights reserved.

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