A Sexually Dimorphic Pattern of Growth Hormone Secretion in the Elderly
P. C. Hindmarsh,
E. Dennison1,
S. M. Pincus,
C. Cooper,
C. H. D. Fall,
D. R. Matthews,
P. J. Pringle and
C. G. D. Brook
London Center for Pediatric Endocrinology, University College
London, London SO16 6YD, United Kingdom; Medical Research Council
Environmental Epidemiology Unit (E.D., C.C., C.H.D.F.), Southampton,
United Kingdom; Guilford (S.M.P.), Connecticut
06437; and Diabetes Research Laboratories, Radcliffe Infirmary
(D.R.M.), Oxford OX2 6HE, United Kingdom
Address all correspondence and requests for reprints to: Dr. P. C. Hindmarsh, Cobbold Laboratories, Middlesex Hospital, Mortimer Street, London, United Kingdom W1N 8AA. E-mail:
p.hindmarsh{at}ucl.ac.uk
In rodents, the sexually dimorphic pattern of pulsatile GH secretionis
an important determinant of growth, liver enzyme functionand
insulin-like growth factor I (IGF-I) expression. Whetherthis
difference is present in humans at different ages is unclear.We
studied GH secretory patterns in the elderly by constructing24-h serum
GH profiles in 45 male and 38 female (age, 59.473.0yr) volunteers
and related patterns to IGF-I, IGF-binding protein-3(IGFBP-3), and
GH-binding protein levels; body mass index; andwaist/hip ratio.
Serum GH concentrations were measured in samples drawn at 20-min
intervalsand analyzed using a sensitive chemiluminescent assay
(NicholsInstitute Diagnostics: sensitivity, 0.036 mU/L).
The 24-h serumGH profiles were analyzed using a concentration
distributionmethod to determine GH peak and trough levels, spectral
analysis,and assessment of serial irregularity by approximate entropy
(ApEn).
There was a highly significant difference in mean 24-h serumGH
concentrations in females compared to males (males, 0.88mU/L; females,
1.31 mU/L; P = 0.009) as a result of significantly
highertrough GH levels (males, 0.04 mU/L; females, 0.16 mU/L;
P <0.001). Peak values were not significantly
different. SerumIGF-I levels were significantly higher in males
(males, 162.4ng/mL; females, 87.8 ng/mL; P <
0.001). Peak GH values wererelated to serum IGF-I levels (males:
r = 0.39; P = 0.009; females:r = 0.5;
P = 0.002), whereas trough GH levels were not.
IGFBP-3levels were similar and related to GH peaks only in males
(r= 0.32; P = 0.03). GH was secreted with a
dominant periodicityof 200 min in males and 280 min in females
(P < 0.025). Theproportion of time taken up by
regular oscillatory activitywas less in females (females, 11.1%;
males, 14.7%; P = 0.01).GH secretion assessed by
ApEn was more disordered in females(males, 0.60; females, 0.81;
P < 0.001), and increasing disorderwas associated
with lower IGF-I levels. Body mass index wasnegatively related to GH
in both sexes. In males, trough valueswere the major determinant
(r = -0.31; P = 0.04), whereas infemales,
the peak value was the major determinant (r = -0.35;
P= 0.04). Trough GH levels were inversely related
in both sexesto waist/hip ratio (males: r = -0.40;
P = 0.006; females: r= -0.44;
P = 0.006) and to increasing secretory disorder
(ApEn;r = -0.46; P < 0.001). These data
demonstrate a sexuallydimorphic pattern of GH secretion in the
elderly.
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