Abstract

Plasma glucocorticoids (GCs) are commonly used as measures of stress in wildlife. A great deal of evidence indicates that only free GC (GC not bound by the specific binding protein, corticosteroid-binding globulin, CBG) leaves the circulation and exerts biological effects on GC-sensitive tissues. Free hormone concentrations are difficult to measure directly, so researchers estimate free GC using two measures: the binding affinity and the binding capacity in plasma. We provide an inexpensive saturation binding method for calculating the binding affinity (equilibrium dissociation constant, K d) of CBG that can be run without specialized laboratory equipment. Given that other plasma proteins, such as albumin, also bind GCs, the method compensates for this non-specific binding. Separation of bound GC from free GC was achieved with dextran-coated charcoal. The method provides repeatable estimates (12% coefficient of variation in the red squirrel, Tamiasciurus hudsonicus), and there is little evidence of inter-individual variation in K d (range 2.0-7.3 nM for 16 Richardson's ground squirrels, Urocitellus richardsonii). The K d values of 28 mammalian species we assessed were mostly clustered around a median of 4 nM, but five species had values between 13 and 61 nM. This pattern may be distinct from birds, for which published values are more tightly distributed (1.5-5.1 nM). The charcoal separation method provides a reliable and robust method for measuring the K d in a wide range of species. It uses basic laboratory equipment to provide rapid results at very low cost. Given the importance of CBG in regulating the biological activity of GCs, this method is a useful tool for physiological ecologists.

Highlights

  • Plasma glucocorticoid (GC) levels are commonly used to assess stress in wildlife

  • We prepare dextran-coated charcoal (DCC) concentrate by adding 100 ml of ultrapure water to 6.25 g of activated charcoal (Sigma, Activated C5260; Norit A) in a graduated cylinder dedicated to charcoal preparation, covering with Parafilm (Pechiney Plastics Packaging, Menasha, WI, USA) and shaking vigorously

  • Most researchers rely on pooled plasma samples when determining Kd, but because there is the potential for inter-individual variation, we decided to measure Kd using individual plasma samples

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Summary

Introduction

Plasma glucocorticoid (GC) levels are commonly used to assess stress in wildlife. most vertebrates have corticosteroid-binding proteins that bind circulating GCs (Seal and Doe, 1965; Desantis et al, 2013), thereby limiting the ability of the GCs to leave the circulation and exert biological effects on tissues. Recent evidence from the biomedical literature supports the proposition that free hormone levels in plasma (i.e. the circulating hormone not bound to orticosteroid-binding globulin, CBG) are what the tissue really ‘sees’ (Qian et al, 2011). Breuner et al, 2013) and that species vary considerably in binding capacity relative to their total plasma GC levels (Desantis et al, 2013), measurement of plasma free hormone levels is essential for understanding the biological significance of GC levels (Breuner et al, 2013). Part of the reason for this may be the perceived difficulty in making the additional measurements needed to quantify free GC concentrations

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