Department of Medicine, Division of Geriatric Medicine, Center on Aging, University of Colorado Health Sciences Center, Denver, Colorado 80262
Submitted 11 November 2002 ; accepted in final form 2 April 2003
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ABSTRACT |
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euglycemic clamp; lipolysis; conjugated estrogens
In postmenopausal women, exogenous hormone replacement has been associated with improved insulin action (10, 16, 18, 26, 38), although this is not a uniform finding (15, 29, 42). Discordant results among clinical studies may be due to variations in hormone treatment (e.g., route of administration, opposition by progestins) or to confounding lifestyle factors (e.g., physical activity, adiposity). The latter possibility is important, because accumulation of adipose tissue after menopause, particularly in the abdominal region, is accelerated and associated with increased risk for glucose intolerance, insulin resistance, and development of type 2 diabetes mellitus (DM) (2, 13, 40, 46). Clinical trials have demonstrated that hormone replacement therapy attenuates age-related increases in abdominal adiposity (i.e., reduced waist size and trunk fat) in postmenopausal women (17, 19, 27). Whether estrogens have an effect on insulin action that is independent of changes in adiposity is unclear. Recent evidence suggests that hormone replacement therapy may reduce the incidence of diabetes by as much as 35% in postmenopausal women (27). Thus elucidating the physiological interactions between sex hormones and insulin action should lead to a better understanding of the progressive risk for type 2 DM in older women.
The purpose of this study was to determine whether whole body insulin action (stimulation of glucose uptake and suppression of lipolysis) is acutely altered by estrogen administration in postmenopausal women. Accordingly, we evaluated glucose infusion rates (GIR) and plasma glycerol concentrations in postmenopausal women during a two-stage hyperinsulinemic euglycemic clamp procedure on two separate occasions, with and without a 2.5-mg intravenous bolus of conjugated estrogens (CE). We hypothesized that raising plasma estradiol to premenopausal midluteal concentrations would acutely improve insulin action in postmenopausal women.
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METHODS |
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Body composition assessment. Total and regional body composition (fat mass and fat-free mass) were determined by dual-energy X-ray absorptiometry using a Lunar DPXIQ (Software v. 4.38; Lunar, Madison, WI). The recommendation of the manufacturer was used to define the trunk region. Waist circumference was measured as the minimum circumference between the top of the iliac crest and the distal end of the rib cage along the midaxillary line.
Aerobic fitness. Maximal oxygen consumption, as an index of aerobic fitness, was measured during exhaustive treadmill exercise using an on-line, open-circuit spirometry system (VMAX; SensorMedics, Yorba Linda, CA).
Glucose disposal. Two-stage (8 and 40 mU · m-2 · min-1) hyperinsulinemic euglycemic clamps were administered according to the methods of DeFronzo et al. (12). Figure 1 illustrates the experimental protocol. For all women, clamps were performed at the General Clinical Research Center (GCRC) after a 12-h fast. An intravenous catheter was placed in an antecubital vein for the infusion of insulin and 20% dextrose. A second catheter was placed retrograde to the venous flow in the contralateral hand for blood sampling. The hand was kept in a warming box that was maintained at 60°C to produce arterialized blood samples (34). After 90 min of baseline measurement, insulin was infused at a constant rate of 8 mU · m-2 · min-1 for 90 min and then increased to 40 mU · m-2 · min-1 for 90 min. Plasma glucose concentrations were measured every 5 min during the insulin infusion by the glucose oxidase method on an automated glucose analyzer (YSI Instruments, Yellow Springs, OH). The dextrose infusion was variably adjusted to maintain plasma glucose at 90 mg/dl. Blood samples were collected at baseline and at 60, 75, and 90 min of each insulin stage for later determination of insulin, estradiol, estrone, catecholamines, free fatty acids (FFA), and glycerol. Whole body GIR were estimated as the steady-state glucose infusion rates (SSGIR) adjusted for fluctuations in plasma glucose concentrations during the final 30 min of each insulin infusion. The clamp procedure was performed on two occasions (in random order) in each woman, with (EST) and without (CON) a 2.5-mg intravenous bolus of CE administered at baseline. Pilot testing revealed that this dose of CE maintained estradiol levels in the premenopausal, midluteal range throughout the duration of the clamp procedure. Five of the women were randomized to receive estrogen at their first study visit, whereas the remaining seven women were randomized to estrogen at their second visit. An average of 4 ± 2 wk separated the 2 testing days.
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Hormones and metabolites. Blood samples were stored at -80°C and analyzed in batches by the Core Laboratory of the GCRC. Serum insulin concentrations were determined with a double-antibody radioimmunoassay (RIA; Pharmacia Upjohn, Kalamazoo, MI). Plasma FFA (Wako Chemicals, Richmond, VA) and glycerol (R-Biopharm, Marshall, MI) were determined enzymatically. Estradiol and estrone were determined by double-antibody RIA (DPC, Los Angeles, CA and DSL, Webster, TX, respectively). Plasma epinephrine (Epi) and norepinephrine (NE) concentrations were determined by HPLC (Dionex DX-500; in-house mobile phase). Intra- and interassay coefficients of variation were as follows: 1) insulin, 5.2 and 9%; 2) FFA, 1.1 and 4.7%; 3) glycerol, 3.4 and 17.3%; 4) estradiol, 6.0 and 11.2%; 5) estrone, 8.7 and 8.6%; 6) Epi, 5.7 and 8.5%; and 7) NE, 4.1 and 7.7%.
Statistics. A two-way repeated-measures ANOVA was used to evaluate
changes in primary outcome variables across the two insulin clamp stages and
between the EST and the CON days. Tukey post hoc comparisons were performed
when a significant day x stage interaction was observed. Main effects
were considered when interaction effects were not significant. Mixed-effects
models were also used to examine the effects of acute intravenous
administration of CE on SSGIR and glycerol concentrations after adjustments
for serum insulin concentrations observed at stages 1 and 2.
Random coefficients for the intercept and slopes were included in the models
to allow for subject-specific effects. When significant day x insulin
interactions were observed, comparisons between the EST and CON days were
performed using least square means at the average serum insulin concentrations
observed across the 2 days during stage 1 (15.6 µU/ml) and
stage 2 (70.8 µU/ml). The main effect of EST was considered when
the interaction term was not statistically significant. Statistical
significance was set at = 0.05. Results are presented as means
± SD unless specified otherwise. All statistical analyses were
performed using SAS software (SAS Institute, Cary, NC).
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RESULTS |
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There was a significant (P < 0.01) day x stage interaction for insulin concentrations such that serum insulin concentrations during stage 1 were not significantly different between EST day (15.1 ± 3.6 µU/ml) and CON day (16.1 ± 4.1 µU/ml) but were significantly lower during stage 2 on the EST day (63.3 ± 12.8 µU/ml) compared with the CON day (78.2 ± 15.8 µU/ml). Despite lower serum insulin concentrations on the EST day, mean SSGIR during stages 1 and 2 were not significantly different between EST day (2.01 ± 0.75 and 7.43 ± 2.42 mg · kg-1 · min-1) and CON day (2.29 ± 0.96 and 7.69 ± 2.54 mg · kg-1 · min-1; Fig. 3A) in the ANOVA model. After serum insulin concentrations in the mixed-effects model were controlled for, SSGIR remained nonsignificantly different between the EST day (2.3 ± 0.9 mg · kg-1 · min-1) and CON day (2.2 ± 1.1 mg · kg-1 · min-1) during stage 1 (mean serum insulin 15.6 µU/ml). However, SSGIR was significantly higher (P = 0.01) on the EST day (8.6 ± 2.5 mg · kg-1 · min-1) than on the CON day (7.2 ± 3.5 mg · kg-1 · min-1) during stage 2 (mean serum insulin 70.8 µU/ml).
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The day x stage interaction for the suppression of glycerol was not statistically significant (P = 0.27) in the ANOVA model. There was a trend (P = 0.09, 40% statistical power) for a main effect of day (i.e., estrogen) on glycerol concentrations such that plasma glycerol tended to be lower during stages 1 and 2 on the EST day (40 ± 16 and 30 ± 7 µmol/l) compared with the CON day (41 ± 16 and 34 ± 11 µmol/l; Fig. 3B). After serum insulin concentrations in the mixed-effects model were controlled for, glycerol levels were not different between the EST day (40 ± 16 µmol/l) and CON day (41 ± 16 µmol/l) during stage 1 (mean serum insulin 15.6 µU/ml) but were significantly lower (P < 0.05) on the EST day (29 ± 7 µmol/l) than on the CON day (35 ± 11 µmol/l) during stage 2 (mean serum insulin 70.8 µU/ml).
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DISCUSSION |
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Ovarian hormones and carbohydrate metabolism. The role of ovarian hormones in glucose and insulin metabolism is unclear. Reduced insulin sensitivity has been observed during the midluteal, compared with the midfollicular, phase of the menstrual cycle (41) as well as during normal pregnancy (24), suggesting that ovarian hormones have a detrimental effect on carbohydrate metabolism. However, both estrogen and progesterone concentrations are elevated during the luteal phase of the menstrual cycle and during late pregnancy, making it difficult to determine the independent effects of these hormones. In the ovariectomized rat model, glucoregulatory action worsens (i.e., insulin resistance) after ovariectomy and is restored with estrogen, but not progesterone, replacement (5, 31). Similarly, insulin action has been shown to be impaired by ovariectomy in nonhuman primates and restored by estrogen-only replacement, but not by progesterone-only or combined estrogen and progesterone replacement (6, 47). Thus the respective roles of estrogens and progestins on carbohydrate metabolism appear to be opposing. In the current study, we acutely administered estrogens to postmenopausal women to determine whether there are acute, independent effects of estrogens on insulin action.
Estrogen replacement and insulin clearance. Prospective, randomized trials have consistently observed reduced fasting insulin concentrations in women treated with hormone replacement compared with those on placebo (4, 79, 16, 18, 20, 45). We (18) and others (4, 10, 32, 36, 45) have observed decreased insulin responses to an oral or intravenous glucose challenge in women treated with hormone replacement. It was not possible in these studies to determine whether the lower insulin levels were due to increased clearance or decreased secretion. However, there is evidence to suggest that estrogens may increase insulin secretion, as C-peptide concentrations increase in response to both oral CE (43) and transdermal estradiol (4, 10). Thus, if the net effect is a reduction in circulating insulin, estrogens must increase insulin clearance to a greater extent than they increase insulin secretion. Cagnacci et al. (4) examined this issue by estimating changes in hepatic insulin clearance from the molar ratio of C-peptide to insulin (fasted and integrated areas during a glucose challenge) in women treated with either transdermal estradiol or oral CE. Treatment with transdermal estradiol resulted in higher C-peptide concentrations but lower fasted and integrated insulin responses, suggesting increased hepatic insulin clearance. An increase in insulin clearance was not observed in response to oral CE. The discordant responses to transdermal and oral estrogen may be related to the first-pass hepatic metabolism effects that occur in response to oral estrogens only. In the present study, we administered CE intravenously, thereby avoiding first-pass hepatic metabolism. Thus effects of intravenous estrogen administration may be more comparable to transdermal than to oral estrogen treatment. Our finding of lower circulating insulin levels in response to the same rate of exogenous insulin infusion on the EST day is consistent with the observation by Cagnacci et al. that hepatic insulin clearance was increased in response to transdermal estrogen therapy.
Previous hormone replacement studies that used the hyperinsulinemic
euglycemic clamp technique
(15,
29,
38) did not observe
significant reductions in either fasted or steady-state insulin concentrations
in women with normal fasted insulin levels. However, two of these studies
(15,
38) reported trends toward
reduced steady-state insulin concentrations after estrogen treatment of
15 to 17%. Furthermore, the effect of estrogens on insulin clearance
measured via the clamp procedure appears to be more robust in hyperinsulinemic
women (3,
10). These findings suggest
that the effects of estrogens on insulin clearance in normoinsulinemic women
are modest and that larger sample sizes are needed for adequate statistical
power. In the present study, we observed an average estrogen-related reduction
in steady-state insulin concentration of 18% during the second stage of the
insulin clamp in relatively normoinsulinemic postmenopausal women. Compared
with previous studies, our improved power to detect a significant effect of
estrogen on insulin concentrations was likely due to our large sample size
combined with a within-subject design to minimize variability. In addition,
unlike previous hormone replacement interventions, we evaluated estrogen
effects on insulin clearance by acutely raising estradiol to the range of
normal for the midluteal phase of the menstrual cycle, thereby improving our
effect size. Although it is not clear whether a reduction in plasma insulin
concentration per se has clinical relevance, the induction of hyperinsulinemia
in rats (30) and humans
(25) has been shown to acutely
alter the action of insulin, including reduced suppression of plasma FFA,
increased de novo lipogenesis, and reduced glucose disposal
(25,
30). Thus it is possible that
an increase in insulin clearance that reduces hyperinsulinemia would itself
contribute to an improved peripheral insulin action.
Estrogen replacement and peripheral insulin action. Estrogen replacement therapies have been shown to increase (3, 10, 18, 38, 43), not change (15, 29) or decrease (42), peripheral insulin action in postmenopausal women. Inconsistency among studies may be due to widely varying types of hormone treatments (e.g., varying duration of treatment, dose, route of administration, and opposition by progestins) and concurrent changes in body composition. Another source of inconsistency among studies may be variation in the methods used to assess insulin action. The prospective, randomized hormone replacement trials that have measured insulin action using the hyperinsulinemic euglycemic clamp technique have demonstrated that insulin-stimulated glucose uptake is not impaired (15, 38) and may be improved (10, 11, 29) by estrogen replacement. Consistent with these previous studies, we observed improvements in the glucoregulatory action of insulin in response to intravenous estrogen administration. Furthermore, our study extends previous observations by assessing the acute physiological effect of estrogen on insulin while eliminating confounding factors such as the first-pass hepatic effects of oral estrogens, opposition by progestins, and changes over time in body composition or physical activity.
Compared with the evidence for an effect of estrogens on glucoregulatory insulin action, the evidence for an effect on antilipolytic insulin action is more consistent. For example, sex differences in lipolysis have been observed such that basal lipolytic rates ([2H5]glycerol rate of appearance) are higher in women compared with men matched for relative adiposity (37). Jensen et al. (26) observed higher FFA release ([14C]palmitate rate of appearance) during a pancreatic clamp in postmenopausal women who had stopped hormone replacement compared with those who had used transdermal estrogen for >2 mo. This estrogen-related attenuation of lipolysis was not explained by changes in Epi stimulation of lipolysis. Additionally, O'Sullivan and Ho (38) observed a reduction in plasma FFA during a hyperinsulinemic clamp in postmenopausal women randomized to transdermal estradiol for 12 wk. This reduction in plasma FFA was not observed in those women randomized to oral CE. Taken together, these data suggest that transdermal estrogen administration has an effect on lipid metabolism that is not catecholamine mediated and may be insulin mediated. Consistent with this possibility, we observed an improvement in the antilipolytic action of insulin (i.e., greater suppression of plasma glycerol) in response to intravenous estrogen administration.
Potential mechanisms. Estrogen receptor-deficient mice and humans are glucose intolerant and hyperinsulinemic (23, 44), suggesting an estrogen receptor-mediated effect on insulin action. Additionally, estrogens may improve insulin action through an increase in specific insulin receptor binding or insulin receptor number (39). However, upregulation of insulin receptors in response to estrogen may be tissue and dose dependent (21, 22). There is further evidence to suggest that estradiol may mimic the action of insulin in adipocytes by activating transcription factors (activator protein-1 and cAMP response element protein) that are also targeted by insulin (14). If estrogens increase adipose tissue insulin sensitivity, particularly in visceral adipose depots drained by the portal circulation, this would be predicted to decrease hepatic FFA flux and increase insulin clearance (1). In the present study, there was no effect of CE on insulin concentrations during the first, low-dose insulin stage as was observed during the second, higher-dose insulin stage. Although the stage-related differences may have been due to a threshold effect (i.e., less insulin to clear), it is also possible that the effects of estrogens on insulin concentrations are indirect and/or time dependent (e.g., through an effect on FFA or upregulation of estrogen receptors). Furthermore, if estrogens increase insulin secretion as well as clearance, the net effect on serum insulin concentration may depend on both the level and the duration of hyperinsulinemia.
Limitations. We cannot rule out the possibility that estrogens had an effect on hepatic glucose production. A study of postmenopausal women with type 2 DM suggested that estrogens might preferentially improve hepatic insulin sensitivity (i.e., more effective suppression of hepatic glucose production) (3). Because we did not assess hepatic glucose production, we do not know whether the SSGIR rates in this study accurately reflected total glucose disposal rates. However, previous research has shown complete suppression of hepatic glucose output between 60 and 120 min, depending on the rate of insulin infusion (28). On the basis of these data, hepatic glucose production should have been nearly completely suppressed during the final 30 min of our first stage, when insulin infusion was low. During the final 30 min of the second stage, when insulin infusion was higher and cumulative insulin exposure had exceeded 150 min, hepatic glucose output should have been completely suppressed, thereby increasing our confidence that SSGIR accurately reflected peripheral glucose disposal.
There is evidence that dose, route, and duration of estrogen administration are important determinants of the effects of hormone replacement therapy on insulin action (10, 32, 33). Our findings may therefore be specific to the intravenous administration of a single 2.5-mg dose of CE that raised plasma estradiol into the premenopausal, midluteal range. Furthermore, we cannot rule out the possibility that estrone or other estrogen metabolites contributed independently or synergistically to the estradiol-related effects on insulin. To our knowledge, this is the first study to measure changes in insulin action in response to acute intravenous estrogen administration.
In summary, acute intravenous administration of CE reduced serum insulin concentrations during a hyperinsulinemic euglycemic clamp, suggesting an increased insulin clearance. After adjustment for the reduced serum insulin concentrations, CE were associated with increased glucose disposal and decreased glycerol concentrations, suggesting enhanced peripheral insulin action. Recent evidence that hormone replacement therapy may reduce the incidence of diabetes by as much as 35% in postmenopausal women (27) highlights the need for future studies to elucidate the mechanisms by which estrogens influence insulin secretion, clearance, and sensitivity.
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DISCLOSURE |
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ACKNOWLEDGMENTS |
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FOOTNOTES |
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The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
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REFERENCES |
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