Abstract
Aim:
Osteocalcin, a biochemical marker of bone formation, has been suggested to be involved in the regulation of energy metabolism. The aim of this study was to investigate the possible association between serum osteocalcin and markers of glucose and lipid metabolism in a large sample of healthy Chinese women.
Methods:
A total of 2032 healthy Chinese women in Shanghai, aged 20–94 (including 1396 discovery-study subjects and 636 postmenopausal women for a reduplication analysis) were recruited. Their serum osteocalcin, calcium and the relevant measurements were analyzed. A Spearman correlation analysis was performed between osteocalcin and the other markers of energy metabolism including triglyceride, total cholesterol, fasting plasma glucose (FPG), serum insulin, body mass index and homeostasis model assessment-insulin resistance. Separate multiple regression analyses were performed with data from the discovery and reduplication subjects to determine whether serum osteocalcin concentration was an independent predictor of the glucose or lipid metabolism markers.
Results:
For the discovery-study subjects, serum osteocalcin was found to be negatively associated with weight (r=−0.08, P=0.002), BMI (−0.13, P<0.001) and FPG (r=−0.13, P=0.001). Similar results were also found in the reduplication subjects (weight: r=−0.19, P=0.016; BMI: r=−0.23, P=0.003; FPG: r=−0.28, P<0.001). In the multiple regression analysis, serum osteocalcin was revealed as a potential independent predictor for FPG (β=−0.07 and –0.210 for discovery and reduplication, respectively, P<0.01) and BMI (β=−0.127 and –0.299 for discovery and reduplication, respectively, P<0.01).
Conclusion:
Serum osteocalcin is negatively associated with weight BMI and FPG in healthy Chinese women. Therefore, osteocalcin might contribute to obesity and diabetes.
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Introduction
Osteocalcin, which is produced and secreted specifically by osteoblasts, is one of the most abundant noncollagen proteins in bone matrix1. Its measurement has been used as a biochemical marker of bone formation and bone turnover2. However, numerous studies have also evaluated the potential role of osteocalcin as a predictor and surrogate marker of fracture risk or osteoporosis3,4. Recent studies have suggested that osteocalcin may also be involved in the regulation of energy metabolism5,6. Lee et al6 demonstrated that mice lacking osteocalcin exhibited hyperglycemia, obesity, decreased β-cell proliferation, glucose intolerance and insulin resistance. Ex vivo studies have found that osteocalcin stimulates the expression and action of CyclinD1, insulin, and adiponectin. Another animal study5, which focused on the mechanism of the novel function of osteocalcin, revealed that mice lacking FoxO1 in osteoblasts had increased pancreatic β-cell proliferation, insulin secretion and insulin sensitivity. FoxO1, which is a member of the Forkhead family of transcription factors, was indicated as a key transcriptional modulator of the endocrine function of the skeleton in regulating glucose metabolism. These findings in mice provided evidence of a novel role of the skeleton in glucose and lipid homeostasis, which is regulated by osteocalcin.
A number of studies have evaluated the complex interactions between the skeleton and glucose and energy homeostasis in humans7,8,9,10,11,12,13,14,15. Osteocalcin was found to be inversely associated with fasting plasma glucose (FPG)7,9,10, HbA1c7,12, body mass index (BMI)10,13, fat mass10, measures of insulin resistance8,14, and measures of lipid metabolism12,15. In these same studies, osteocalcin was positively associated with adiponectin11 and measures of insulin sensitivity7,15. Among these studies, the positive relationship between osteocalcin and markers of metabolic phenotype were revealed mostly in the elderly population or subjects with diabetes mellitus. Recently, a study found that serum osteocalcin levels were inversely correlated with visceral fat area in Chinese men16. However, the results of the studies on the association between osteocalcin and lipid metabolism are inconsistent7,13,15. Therefore, it is necessary to perform more human osteocalcin-metabolism association studies with larger sample sizes and healthy populations to provide insights into the relation between serum osteocalcin levels and glucose and lipid metabolism.
In this study, we performed a cross-sectional analysis to investigate the possible association between osteocalcin and markers of glucose and lipid metabolism in a large sample of healthy Chinese females.
Materials and methods
Subjects
The study was approved by the Ethics Committee of the Shanghai Jiao Tong University Affiliated Sixth People's Hospital. Between February and March 2009, we recruited 2243 women (aged 20–96 years) living in Shanghai from several community centers. But only 1396 people can independently complete the questionnaire and physical examination. Of these 1396 women, 39 failed the initial screening, leaving 1357 subjects with detected serum osteocalcin. All the subjects belonged to the Chinese Han ethnic group and signed informed consent documents before entering the study17. All subjects completed a questionnaire, providing information on age, medical history, etc. A physical checkup and routine serum examination were performed. All of the subjects were found to be in good health. None of the subjects suffered from diseases known to affect bone metabolism or used drugs affecting bone metabolism. Subjects who had a history of diabetes mellitus or fasting plasma glucose (FPG)>7.0 mmol/L were not eligible for the study.
For the reduplication analysis, 636 healthy ambulatory postmenopausal women (aged 55–75 years) were recruited for a national clinical trial on the prevention of bone fracture in a population with a high risk of osteoporosis. The exclusion criteria were the same as in our previous study, including the presence of the following: (1) serious residual effects from cerebral vascular disease; (2) diabetes mellitus; (3) hyperthyroidism; (4) chronic renal disease or renal lithiasis; (5) serious chronic liver disease; (6) significant chronic gastrointestinal disease; (7) rheumatoid arthritis or collagen disease; (8) cancer; (9) corticosteroid or anticoagulation therapy at pharmacological levels; (10) evidence of other metabolic or inherited bone diseases; (11) treatment with calcium>600 mg/d or VitD>600 IU/d; (12) therapy with bisphosphonate or fluoride in the past 1 year; or (13) therapy with calcitonin, estrogen or SERMs in the past 3 years18.
Blood measurement
The blood samples were collected after an 8-h or greater overnight fast for measurement of serum calcium (Ca), phosphate (P), alkaline phosphatase (ALP), triglyceride (TG), total cholesterol (TC), and fasting plasma glucose (FPG). The electrochemiluminescence immunoassay (ECLIA, Elecsys autoanalyzer, Roche Diagnostics GmbH, Germany) was used to measure the serum insulin (intra and inter assay coefficients of variation of 1.5%–2.0% and 2.1%–2.8%, respectively). Serum 25-hydroxyvitamin D [25(OH)D], parathyroid hormone (PTH), β-cross-linked C-telopeptide of type l collagen (CTX), osteocalcin in form of N-MID, and N-terminal procollagen of type l collagen (P1NP) were measured using an automated Roche electro-chemiluminescence system (Roche Diagnostic Gmbh, Germany). The intra- and inter-assay coefficients of variation (CVs) for 25(OH)D were 5.6% and 8.0%, respectively. The lower limit of detection for 25(OH)D was 4 ng/mL (10 mmol/L). The intra- and interassay CVs were 1.4% and 2.9% for PTH, 2.5% and 3.5% for β-CTX, 2.9% and 4.0% for osteocalcin, and 2.3% and 2.8% for P1NP, respectively17,19,20.
Other measurements
A physical examination including the measurement of height and weight was performed for each participant. Body mass index (BMI) was calculated as weight divided by squared height (kg/m2). The assessment of insulin sensitivity was estimated by homeostasis model assessment-insulin resistance (HOMA-IR) based on FPG and insulin measurements as follows: HOMA-IR=[fasting serum insulin (mU/L)×FPG (mmol/L)]/22.514.
Statistical analysis
All statistical analyses were performed using SPSS version 19 software (SPSS Inc of IBM, USA). Skewed variables were transformed to natural logarithms for the formal analyses. The ANOVA test was used to compare the general characteristics between the quartiles of serum osteocalcin. Spearman correlation analysis was performed between osteocalcin and the other factors; the Spearman correlation coefficients for the glucose, lipid and bone metabolism parameters were calculated to determine which factors would be included in the final model (data not shown). In the final model, multivariate regression analysis was performed to determine the associations between serum osteocalcin as the independent variable and FPG, insulin, HOMA-IR, TG, TC, and BMI after adjusting for age, BMI, Ca, P, ALP, TG, TC, and PTH (No adjustment was made for BMI, TG, or TC when they were included as outcome variables in the model).
In the 636 postmenopausal female subjects included as reduplicated samples, the spearman correlation and multivariate regression analysis were repeated to compare against the results from the discovery study. For all statistical analyses, P<0.05 was considered significant.
Results
The clinical characteristics of the study subjects
Among the 1396 female participants of the discovery study, 39 women who met the exclusion criteria were removed from the analysis. The general characteristics of the subjects in the discovery study and the reduplication group were summarized in Table 1. For the reduplication analysis, the mean age, BMI, and FPG of 636 healthy postmenopausal women were 62.8±5.8 year, 24.7±3.3 kg/m2, and 4.74±0.59 mmol/L, respectively.
The discovery study subjects were divided into quartiles by their serum osteocalcin concentration (Table 2). BMI varied inversely with the osteocalcin quartiles (P<0.01). The FPG level in the lowest osteocalcin quartiles was significantly higher than in the other quartiles in both the pair-wise and overall comparisons. No significant differences or tendencies in the serum insulin, HOMA-IR, TG, or TC were found according to the quartiles of osteocalcin.
The correlation between serum osteocalcin and other para-meters
We studied the association between serum osteocalcin and other body or serum/plasma parameters in both the discovery study and the reduplication subjects (Table 3). For the discovery study subjects, serum osteocalcin was negatively associated with weight, BMI and FPG (r=−0.08, r=−0.13, and r=−0.13, respectively, P<0.01); the negative associations with weight, BMI and FPG were also found in the reduplication subjects (r=−0.19, r=−0.23, and r=−0.28, respectively, P<0.05). The correlation was significantly stronger between serum osteocalcin and FPG in the postmenopausal women than in the overall group containing both young and elderly subjects (r=−0.28 and r=−0.13, P<0.01). However, no significant association between serum osteocalcin and insulin/HOMA-IR was detected in either the discovery or the reduplication groups. Furthermore, no association was found between the two markers of lipid metabolism, TG and TC, and serum osteocalcin in the discovery study subjects.
The multiple regression analyses for osteocalcin as the inde-pendent predictor
To determine whether the serum osteocalcin concentration was an independent predictor of the markers of glucose or lipid metabolism, we performed separate multiple regression analyses in the discovery and reduplication subjects (Table 4). In the discovery subjects, we found a negative association between serum osteocalcin and FPG after adjusting for age, BMI, Ca, P, ALP, PTH, TG, and TC (β=−0.07, P<0.01). Also a negative association between serum osteocalcin and BMI was found after adjusting for age, FPG, Ca, P, ALP, PTH, TG, and TC (β=−0.127, P<0.01). Serum osteocalcin levels were also inversely associated with FPG and BMI (β=−0.210 and β=−0.299, P<0.01) in the reduplication study. However, no evidence was found that serum osteocalcin played a role as an independent predictor of serum insulin, HOMA-IR, TG, or TC in either the discovery or the reduplication subjects.
Discussion
Osteocalcin, which contains 49 amino acids (including 3 γ-carboxylated glutamic acid residues), is produced and excreted by osteoblasts21,22. As a classic biochemical marker for bone turnover, the circulating osteocalcin has been measured widely in the diagnosis and treatment of metabolic bone diseases23. However, recent studies have suggested that osteocalcin may also be involved in the regulation of energy metabolism. Lee et al6 showed that mice lacking the osteotesticular protein tyrosine phosphatase (OST-PTP) were hypoglycemic and were protected from obesity and glucose intolerance. OST-PTP, which is encoded by the enterococcal surface protein gene (Esp), has been found to downregulate the activity of osteocalcin24.
In the present study, we revealed that serum osteocalcin was negatively associated with BMI in Chinese healthy women. The mechanisms associating fat mass with osteocalcin are not fully understood. It has been suggested that osteocalcin concentrations are modulated by the adipocytokine leptin. In humans, lower circulating osteocalcin levels were found in overweight25 and diabetic subjects26 compared with normal weight individuals.
In our study, we also found a negative association, which was also confirmed in the reduplication analysis, between serum osteocalcin and BMI, which was a phenotype of obesity. In a previous study, Bao et al16 also found that visceral fat area and percent body fat were independent factors negatively associated with serum osteocalcin levels in Chinese men. In animal studies, after 6 weeks of a high-fat diet, the body weight of the Esp−/− mice increased at a slower rate than did the wild type (WT) mouse6. In another mouse model, the Ocn−/− mouse, in which the Osteocalcin gene was knocked out, was obese and had significantly increased fat mass and numbers of adipocytes. The results of our study are in agreement with others who have shown the inverse association between osteocalcin and BMI. However, in addition to BMI, fat mass and lean mass, which are measured by dual energy x-ray absorptiometry (DXA), are also useful markers reflecting body composition and obesity. It is unfortunate that we were not able to test fat mass and lean mass by DXA to further confirm the association between serum osteocalcin and the phenotypes of obesity in this population. However, a recent study found that visceral fat area was inversely associated with serum osteocalcin levels in Chinese men, which is in agreement with our results16.
A significantly lower osteocalcin concentration has been found in patients with diabetes mellitus than in healthy individuals27,28,29; this phenomenon may be the result of a decrease in the number of osteoblasts due to hyperglycemia30,31. However, according to Lee et al's study6, osteocalcin may also regulate glucose metabolism. Previous studies in humans have attempted to reveal the relationship between osteocalcin and glucose metabolism7,8,9,10,12,14,15. In the present study, we revealed that serum osteocalcin was negatively associated with FPG. However, we found no further evidence to support the theory that total serum osteocalcin plays a role as an independent predictor of the phenotypes of insulin resistance in either the discovery or reduplication subjects. Our results are similar to that of a study of elderly Swedish men10, in which Kindblom et al found that plasma osteocalcin was inversely related to the plasma glucose, not insulin resistance.
Based on the limited number of existing studies, the relationship between osteocalcin and lipid metabolism in humans remains unclear. In the present study, we analyzed the independent impact of osteocalcin on two phenotypes of lipid metabolism, TG and TC, in the discovery subjects. No association was found to prove that osteocalcin affected these two markers of lipid metabolism. In the previous human studies, Im et al13 failed to find an association between serum osteocalcin and blood lipids in postmenopausal women, and Zhou et al7 revealed that serum osteocalcin was positively associated with high-density lipoprotein cholesterol in Chinese elderly men and TG in premenopausal women. The current study conducted in a large sample of the healthy population provides useful data on the relationship between osteocalcin and lipid metabolism in humans.
The results of the present study suggest that circulating osteocalcin is involved in the regulation of obesity and blood glucose, but not in the regulation of insulin resistance and lipid metabolism. Previous studies have found increased insulin sensitivity in the Esp−/− mouse suggesting that circulating osteocalcin enhances insulin sensitivity through the increased expression of adiponectin6,32. Adiponectin is a polypeptide which modulates glucose regulation and fatty acid catabolism33. It has been reported that adiponectin concentration is inversely correlated with body fat percentage in adults34. Recently, adiponectin was also shown to have a positive association with serum osteocalcin in postmenopausal women with diabetes mellitus. We investigated the relationship between osteocalcin and insulin resistance by calculating the subject's HOMA-IR, which was found to be inversely associated with serum osteocalcin in the previous studies9. Our negative results may reflect the imprecision of HOMA-IR as a surrogate measure of insulin resistance. The detection of the adiponectin concentration would have helped further elucidate the relationship between osteocalcin and insulin resistance in this study.
The further study of the mechanism of osteocalcin's regulation of insulin resistance may contribute to the treatment of a series of energy metabolism diseases. A recent animal study5 showed that mice lacking Foxo1 only in osteoblasts had increased pancreatic β-cell proliferation, insulin secretion and insulin sensitivity. Foxo1 was indicated to be an upstream regulator that controls glucose metabolism through the stimulation of osteocalcin and the inhibition of Esp expression in osteoblasts.
On the other hand, all of the animal studies provide evidence that only uncarboxylated osteocalcin influences energy metabolism in mice6,32. Nevertheless, osteocalcin is only able to bind calcium in its carboxylated form, which depends on vitamin K and carbon dioxide. In women, (elevated/decreased) uncarboxylated osteocalcin levels were found to be a risk factor for bone fracture35 and were associated with a (increase or decrease) in vitamin K levels. This research suggests that uncarboxylated osteocalcin plays an adverse role in bone metabolism and energy metabolism. Further study of the maximally-beneficial level of circulating osteocalcin should be performed in the future.
The present study has several limitations. Our measurement of osteocalcin was N-mid osteocalcin, which cannot be separated into its carboxylated and uncarboxylated forms. Additional markers of the phenotypes of energy metabolism such as HbA1c, fat mass, and lean mass were not investigated in this study. The present study used a cross-sectional design with healthy subjects; it is necessary for us to perform a long-term prospective analysis to confirm the study results.
However, the present study still revealed valuable information about the association between osteocalcin and energy metabolism. In a large sample of the healthy Chinese population, we found that the serum osteocalcin concentration was inversely associated with plasma glucose and was a strong predictor of BMI; these results were also confirmed in postmenopausal Chinese women as a reduplication analysis. Our data supported the finding that osteocalcin is involved in the regulation of energy metabolism. Therefore, osteocalcin might be a promising link between obesity and diabetes.
Author contribution
Wei-wei HU designed the study, carried out all statistical analyses and drafted the manuscript. Zhen-lin ZHANG conceived and designed the study and revised the manuscript. Di CHEN revised the manuscript. Jin-wei HE guided the work of the genetics laboratory and guaranteed and confirmed the quality of the genetic data. Wen-zhen FU guided the work of the genetics laboratory. Yao-hua KE carried out the field-work including sample and data collection. Yu-juan LIU coordinated the DNA sample collection. All authors read and approved the final manuscript.
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Acknowledgements
This study was supported by the National Natural Science Foundation of China (NSFC) (Grant Nos 81370978, 81070692 and 81170803), Academic Leaders in Health Sciences in Shanghai (XBR2011014), 2014CB942903, SHDC12013115, CSTC2013jcyjC00009, National Basic Research Program of China (Grant No 2014CB942903 to Zhen-lin ZHANG) and Program for Outstanding Medical Academic Leader (051).
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Hu, Ww., Ke, Yh., He, Jw. et al. Serum osteocalcin levels are inversely associated with plasma glucose and body mass index in healthy Chinese women. Acta Pharmacol Sin 35, 1521–1526 (2014). https://doi.org/10.1038/aps.2014.92
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DOI: https://doi.org/10.1038/aps.2014.92
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