The Relationship between Follicle-stimulating Hormone and Bone Health: Alternative Explanation for Bone Loss beyond Oestrogen?

Bone loss in women commences before the onset of menopause and oestrogen deficiency. The increase of follicle-stimulating hormone (FSH) precedes oestrogen decline and may be a cause for bone loss before menopause. This review summarizes the current evidence on the relationship between FSH and bone derived from cellular, animal and human studies. Cellular studies found that FSH receptor (FSHR) was present on osteoclasts, osteoclast precursors and mesenchymal stem cells but not osteoblasts. FSH promoted osteoclast differentiation, activity and survival but exerted negligible effects on osteoblasts. Transgenic FSHR or FSH knockout rodents showed heterogenous skeletal phenotypes. Supplementation of FSH enhanced bone deterioration and blocking of FSH action protected bone of rodents. Human epidemiological studies revealed a negative relationship between FSH and bone health in perimenopausal women and elderly men but the association was attenuated in postmenopausal women. In conclusion, FSH may have a direct action on bone health independent of oestrogen by enhancing bone resorption. Its effects may be attenuated in the presence of overt sex hormone deficiency. More longitudinal studies pertaining to the effects of FSH on bone health, especially on fracture risk, should be conducted to validate this speculation.

Introduction

Accelerated bone loss in women during menopausal transition is often attributed to oestrogen deficiency. However, the Study of Women's Health Across the Nation (SWAN) involving women from various ethnic groups showed negligible changes in the bone mineral density (BMD) in pre- and early perimenopausal women. Significant bone loss was observed in late perimenopausal women (0.018 and 0.010 g/cm2 yearly at the spine and hip) and the rate increased in postmenopausal women (0.022 and 0.013 g/cm2 yearly at the spine and hip) 1. On the other hand, the decline of oestrogen level transpires very late during perimenopause but the gonadotropin levels, especially follicle-stimulating hormone (FSH), gradually increase 5-6 years before menopause 2, 3. Thus, oestrogen deficiency alone may not explain the accelerated bone loss during this period.

Although ovariectomy in female rodents invariably causes a reduction in bone mass, studies that inhibit the function or knockout the oestrogen receptors (ERs) in rodents showed contradictory results. Ogawa et al. (2000) generated a rat model with a dominant negative ERα which inhibited both ERα and ERβ. The transgenic rats showed similar BMD with the wildtypes. After ovariectomy, the transgenic rats also showed a similar degree of bone loss compared with the wildtype, and the condition could not be reversed with oestrogen replacement 4. In another study, ERβ knockout female mice showed increased bone mineral content at the cortical bone compared to the wildtype at 11 weeks old, as well as increased trabecular BMD and bone volume at 1 year old. The ERβ knockout male mice showed similar skeletal phenotypes as the wildtype 5, 6. The importance of oestrogen in maintaining bone health was further complicated by the fact that hypophysectomy inhibited high bone turnover induced by ovariectomy in rats 7. Subsequently, Sun et al. (2006) observed that FSH receptor (FSHR) knockout mice maintained their bone health despite being hypogonadal 8. Despite receiving criticisms on the model used, their research raised the question whether FSH plays a more vital role in regulating bone loss among women during menopause transition period.

The controversy on the role of FSH on bone metabolism remains to-date. The studies aforementioned hint a negative impact of high FSH on bone health. However, sex hormone deprivation therapy using gonadotropin agonists for the treatment of prostate cancer has been shown to induce bone loss in animals and humans 9-11. Most importantly, oestrogen-centric therapies, such as hormone replacement therapy and selective oestrogen receptor modulator, have been successful in treating postmenopausal osteoporosis and preventing fractures 12-14. Considering the complexity of this issue, this review aims to summarize the current evidence on the skeletal effects of FSH from cellular, animal and human studies. This issue is relevant because it can potentially shift the paradigm of an oestrogen-centric explanation for bone loss during menopause transition period. It may also offer a new avenue for the treatment of postmenopausal bone loss.

Mechanism of FSH action on bone cells

Protein and mRNA expression of FSHR have been detected in human monocytic cells (sharing the same lineage with osteoclast), osteoclasts and mesenchymal stem cells at a concentration lower than in ovarian samples 8, 15. However, they were absent in human osteoblasts 15. The FSHR expressed in these cells belonged to the type-2 FSHR isoform and the expression level was not influenced by sex hormones 15. The blocking of FSHR with mono- or polyclonal antibodies abolished the formation of osteoclast-like cells from bone marrow macrophages from mice 16. Similarly, the promoting effects of FSH on osteoclast formation was impaired in bone marrow macrophages from FSHR knockout mice 16. These studies showed that FSHR is essential for the action of FSH in promoting osteoclast formation.

Sun et al. (2006) showed that FSH increased osteoclast differentiation in human peripheral blood macrophages, mouse bone marrow culture and RAW cells but did not influence the proliferation of osteoclast precursors directly 8. On the other hand, FSH induced the production of tumour necrosis alpha (TNFα) in monocytes and bone marrow macrophages from mice 15, 17, which in turn promoted the proliferation of osteoclast precursor cells as illustrated in cellular and in silico studies 17. Several pathways related to osteoclast formation in monocytes were activated by FSH, including osteoclast differentiation (toll-like receptor and interleukin-1 receptor-associated kinases), cell adhesion, survival (anti-apoptotic TNFs/nuclear factor-κB/B-cell lymphoma 2 (BCL-2)) and cytoskeletal remodelling 15. FSH promoted the formation of tartrate-resistant acid phosphatase (TRAP) positive cells (osteoclast-like cells) from various types of macrophages (RAW 264.7 cells, RAW c3 cells, bone marrow macrophages from mouse) through FSHR 18. This process was mediated by the ability of FSH to activate pathways essential to osteoclastogenesis, such as phosphorylation of protein kinase B (Akt) and extracellular-signal-regulated kinase (Erk), and nuclear translation of c-fos 18. FSH also increased the formation of resorption pits and action ring of osteoclast-like cells, as well as promoted their survival 18. This corroborated with the findings of Robinson et al. (2010) 15. In short, FSH increases the proliferation of osteoclast precursors indirectly through inflammatory cytokines, as well as their differentiation into mature osteoclasts through direct interaction with the signalling pathways involved. Furthermore, it also promotes the bone resorption activity of osteoclasts.

Apart from TNFα, osteoclast formation also requires the interaction between receptor activator of nuclear factor κ-Β (RANK) on osteoclast surface and RANK ligand (RANKL) secreted by osteoblast. Cannon et al. (2011) showed that FSH at 50 mIU/ml (physiological FSH level in perimenopausal women) promoted the expression of RANK on human CD14+ monocytes 19. However, at 100 mIU/ml (physiological FSH level in postmenopausal women), the effect of FSH was attenuated 19. Similarly, Wang et al. (2015) found that with increasing concentration of FSH, the mRNA expression of RANK increased concurrently with other markers of osteoclast differentiation (TRAP, MMP-9 and cathepsin K) in RAW 264.7 cells 20. Thus, FSH-induced osteoclastogenesis may be a result of increased RANKL-RANK interaction.

Conversely, negative results on the effects of FSH on osteoclast formation have also been reported. Ritter et al. (2008) showed that FSH did not affect the resorption pit area and formation of osteoclasts from human mononuclear cells and RAW cells 21. However, at 3 µg/ml, FSH decreased the formation of multinucleated TRAP-positive cells 21. FSH also did not affect the gene expression of osteoclast markers, such as TRAP, calcitonin, MMP-9, aquaporin 9, V0ATPase, TRAF6 and FSHR. The concentration difference could contribute to the discrepancy of this study with the previous ones 21.

Sun et al. (2006) showed that FSH did not influence the formation of mineralized nodules by colony forming units in mice bone marrow culture. It also did not affect the synthesis of RANKL 8. This was not surprising since FSHR was absent in osteoblasts. Since mesenchymal stem cells displayed FSHR and the differentiation of osteoclasts required soluble factors from other cells, the indirect action of FSH in promoting osteoclastogenesis was tested. Sun et al. (2006) found that coculturing stromal cells, which was supposed to produce factors stimulating osteoclast formation, with FSHR-/- macrophages in the addition of FSH did not stimulate osteoclastogenesis 8. Considering all evidence above, the effects of FSH on osteoclast formation is direct, without the involvement of osteoblasts or stromal cells.

Despite the absence of FSHR and the lack of effects in osteoblasts, FSH could enhance the osteogenic potential of mouse embryonic fibroblasts, indicated by increased bone morphogenetic protein 9 (BMP-9) and alkaline phosphatase activity 22. Combination of FSH and BMP-9 transfection increased the protein and mRNA expression of osteoblast markers (osteopontin and osteocalcin) and matrix mineralization in embryonic fibroblasts 22. This was mediated by increased phosphorylation Smad1/5/8 and expression of transcription factors osterix and runt-related factor-2 essential in osteoblast formation 22. When the transfected cells were injected into the flank of nude mice, they formed a bony mass 22. Although being an innovative therapeutic approach, the use of genetically manipulated fibroblasts prevents the interpretation of FSH action on bone formation in normal physiology.

Therefore, the FSH seems to exert a direct effect on osteoclasts by promoting their formation, resorption activity and survival through FSHR. FSH enhances the osteogenic potential of pluripotent stem cells but its action on osteoblasts remains unclear due to the absence of FSHR in osteoblasts (Figure 1).

Figure 1

The direct effects of FSH on bone cells. FSH increases the expression of RANK and production of TNFα by osteoclast precursors. It also enhanced pathways leading to osteoclast differentiation. Formation of actin ring and resorption pits increase with FSH. It also prevents the apoptosis of osteoclasts. The effects of FSH on osteoblasts are not clear. Abbreviation: Akt=protein kinase B; c-FOS=Fos proto-oncogene; Erk=extracellular-signal-regulated kinase; FSH=follicle-stimulating hormone; MMP-9=matrix metallopeptidase 9; OPG=osteoprotegerin; RANK=receptor activator of nuclear kactor κ B; RANKL= RANK ligand

Animal studies

Sun et al. (2006) piloted the study on the skeletal effects of FSH using FSHR knockout (FSHR-/-) female mice 8. These mice were hypogonadal but their bone status in terms of areal BMD, femoral trabecular microstructure and bone remodelling markers were similar with the wildtype mice 8. This showed that eliminating the interaction between FSH and bone protected bone health in these hypogonadal mice. Culture of calvarial bone extracted from mice showed that FSH and RANKL enhanced formation of TRAP-positive surface in wildtype samples but not in FSHR-/- samples 8. This observation was in accordance with the in vitro osteoclast generation assays using macrophages. FSHβ knockout mice (FSHβ-/-) shared similar skeletal features with FSHR-/- mice. On the other hand, FSHβ haploinsufficient (FSHβ+/-) female mice, which were eugonadal, had a higher femoral BMD but similar lumbar spine, femoral neck and tibial BMD compared with the wildtype and FSHβ-/- mice 8. Femoral cortical thickness and trabecular structural indices were higher in the FSHβ+/- mice compared to the wildtype 8. This was expected since the presence of oestrogen and the attenuated FSH interaction provided protections to the bone of these mice. TRAP-labelled resorption surfaces and serum TRAP level were reduced in the FSHβ+/- mice but mineralising surface and mineral apposition rate were similar in both the FSHβ+/- mice and the wildtype mice 8. mRNA expression of TRAP, cathepsin K and RANK were reduced in the bone marrow of FSHβ+/- mice compared to wildtype 8. This reflects a reduced osteoclast differentiation in the bone of these mice. This study received criticism for overlooking the fact that FSHR-/- female mice had very high testosterone level, which could be accountable for the observed bone-sparing phenomenon 23. The increased testosterone level was due to the double negative feedback actions, whereby the pituitary synthesised higher LH level in the absence of FSH, which in turn increased the production of testosterone by theca cells in the ovaries. As a result, raised testosterone level and uterine degeneration had been observed in FSHR-/- mice 23-25. Hence, the use of transgenic animals cannot fully resolve the skeletal action of FSH due to changes in the hormonal milieu.

By contrast, Gao et al. (2007) showed that FSHR-/- mice demonstrated lower femoral and lumbar spine BMD values starting from month three of age compared to wildtype 26. The trabecular bone volume, osteoblast number, bone formation rate and mineral apposition rate were also lower in these mice compared to the wildtype 26. Concurrently, osteoclast number, RANKL/OPG number were significantly higher in FSHR-/- mice compared to the wildtype 26. The cause of these degenerative bone changes was oestrogen deficiency, as ovarian transplantation prevented the decline in BMD 26. The high testosterone level apparently did not prevent bone loss in the FSHR-/- mice. Ovariectomy reduced BMD and trabecular bone volume, as well as increased osteoclast surface and RANKL/OPG ratio in both FSHR-/- and wildtype mice, but only osteoblast surface, mineralizing surface and bone formation rate increased in wildtype mice, indicating a higher bone turnover level 26. The lack of osteoblastic response in FSHR-/- mice might suggest the uncoupling of bone remodelling process, although previous studies had established that FSH might not possess direct effects on osteoblasts 8. Ovariectomy also eliminated the high circulating testosterone level in the mice 26. Blocking the effects of testosterone using flutamide did not reduce the BMD in FSHR-/- mice, but blocking the conversion of testosterone to oestrogen using letrozole, an aromatase inhibitor, did 26. Flutamide did reduce the trabecular bone volume and increase osteoclast surface in the mice, while letrozole increased osteoclast surface and reduced osteoblast surface and bone formation rate 26. This illustrated that oestrogen might be more important than testosterone in determining the bone health of FSHR-/- mice 26.

By using transgenic mice expressing human FSH independent of the pituitary (TgFSH) with or without hypogonadism, Allan et al. (2010) showed that higher FSH level was associated with higher tibial and vertebral bone volume regardless of gonadal status 27. This observation was different from the previous study that pointed to the skeletal degenerative effects of FSH. The phenomenon might be contributed by the high testosterone and inhibin A level in FSH-high-expression mice 27. Very high FSH also caused the formation of woven bone in marrow space and increased osteoblast surface 27. This was not shown in TgFSH mice with moderate FSH level 27. The results suggest that the skeletal effects of FSH, at least on bone formation, were concentration dependent. However, the osteoclast surface was similar across high FSH, moderate FSH and wildtype mice 27. Hypogonadal TgFSH mice showed reduced N-terminal propeptide of type I procollagen (PINP) and increased TRAP, indicative of an imbalanced bone remodelling towards bone resorption 27. Non-hypogonadal TgFSH mice expressing high FSH also showed higher TRAP level 27. Ovariectomy abolished the skeletal protective effects of FSH in the hypogonadal group, indicated by reduced bone volume, reduced TRAP and PINP 27. This showed that an intact ovary was needed for the skeletal action of FSH.

Apart from genetically modified mice, supplementation of FSH on normal rodents has also been used to examine the effects the hormone on bone. Liu et al. (2010) supplemented 3 µg/kg FSH for two weeks to ovariectomized rats aged 3-4 months with periodontitis 28. FSH increased alveolar bone loss in ovariectomized rats with periodontitis, as evidenced by increased distanced between amelocemental junction to alveolar crest, compared to untreated rats 28. The osteoclast number at the bone crest of furcation region was increased in rats with periodontitis treated with FSH compared to untreated rats 28. Immunohistological staining showed that the number of FSHR positive cells correlated positively with alveolar bone loss area 28. Therefore, this study shows that high FSH aggravates bone loss in rats with pre-existing inflammatory condition.

Lukefahr et al. (2012) used 4-vinylcyclohexene diepoxide (VCD) to establish a hormonal milieu similar with premenopausal women (high FSH, normal oestrogen) in rats 29. Distal femoral BMD was lower in VCD-treated rats starting from two months and 11 months after treatment of 160 and 80 mg/kg/day VCD was initiated 29. This corresponded to the changes in their hormonal milieu, whereby FSH increased consistently two months after treatment initiation in VCD-treated rats 29. Their oestrogen level was similar with the untreated rats 29. Correlation studies revealed a negative relationship between distal femoral BMD and FSH 29. Therefore, this study validates that high FSH is detrimental to bone health in the presence of normal oestrogen level. However, the model used in this study might not resemble postmenopausal women entirely because the circulating inhibin A level was suppressed in VCD-treated rats but it did not happen in women undergoing menopausal transition 29.

The skeletal effects of FSH could be also illustrated by blocking its action using an antibody. Geng et al. (2013) immunized three-month-old ovariectomized rats with FSHβ antibody 30. Three months later, they found that femoral BMD, trabecular structural indices (bone volume, thickness and number) and biomechanical indices (maximum load, stiffness, Young's modulus and stress) were significantly higher in the immunized ovariectomized rats than untreated rats 30. Therefore, blocking the effects of FSH could partially eliminate some of the negative skeletal changes of hypogonadism in these rats.

Only one supplementation study revealed a negligible association between FSH and bone health. Ritter et al. (2008) supplemented 16-week-old male mice with 6 or 60 µg/kg/day FSH intermittently or 6 µg/kg/day continuously via osmotic pump for one month. FSH did not alter the femoral BMD or any trabecular indices in the mice 21. It is unclear whether the skeleton of normal male mice is less responsive of the effects of high FSH compared to female mice.

Human studies

Premenopausal Women

Many observational studies on the relationship between FSH and bone health among premenopausal women have been performed. Among 68 spontaneously menstruating women aged 45-55 years, Garton et al. (1996) showed that those with FSH level at the highest tertile (>35 IU/l) had the lowest lumbar spine and femoral BMD, lowest forearm trabecular bone density assessed by peripheral quantitative computed tomography (pQCT), and the highest serum phosphate, pyridinoline (PYD) and deoxypyridinoline (DPD) level 31. Similarly, Cannon et al. (2010) demonstrated that FSH was the significant negative predictor of total BMD and lumbar spine BMD among 36 women aged 20-50 years with normal menstrual cycles, after adjustment for confounding factor such as oestrogenic hormones, inhibin-B, age, body anthropometry and leisure time physical activity 32. Both studies were limited by their small sample size. Using the data from SWAN, a large multiethnicity (Caucasian, African American, Japanese, Chinese) involving 2336 women aged 42-52 years, Sowers et al. (2003) found that the relationships between FSH and femoral neck, total hip and lumbar spine BMD were negative, independent of ethnicity, physical activity and BMI of the subjects 33. In the subsequent analysis, Sowers et al. (2003) found that a higher FSH was associated with a higher N-terminal telopeptide (NTX) level and a lower osteocalcin level. Other sex hormones were not associated with the variation in bone remodelling markers 34. The relationship between FSH and BMD at three different phases of menses (ovulatory, anovulatory and ovulatory disturbance) was also re-examined in a subset of SWAN subjects consisting only of African American and Caucasian women (n=643, aged 43-53 years). Urinary FSH was negatively and significantly associated with lumbar spine BMD at all three phases 35. Therefore, higher FSH is associated with poorer bone health indicated by BMD and higher bone resorption indicated by bone markers, among premenopausal women as evidenced in these studies.

The association between bone health and FSH suggested by cross-sectional studies is hypothetical at best because the causal relationship cannot be assessed. Therefore, longitudinal studies were performed to validate this relationship. Among 130 non-Hispanic Caucasian women aged 31-50 years followed up for 1-9 years, Hui et al. (2002) revealed that those who lost bone faster (>1% BMD reduction per year) had significant higher FSH and LH, and lower oestradiol compared to those who lost bone slower 36. The rate of bone loss was inversely associated with FSH level in all subjects regardless of BMD value 36. The study was restricted by its sample size and the wide variation in follow-up period. Data from SWAN (n=2311) showed that the degree of bone loss over 4 years was related with the baseline FSH level in the subjects 37. Those with a baseline FSH < 25 mIU/ml lost 0.05 g/cm2 lumbar spine BMD when their follow up FSH raised to 40-70 mIU/ml. Those with a higher baseline FSH (35-45 mIU/ml) lost similar amount of BMD when their follow-up FSH raised to 40-50 mIU/ml. The greatest lumbar spine BMD loss (0.069 g/cm2) occurred when the follow up FSH level was 70-75 mIU/ml 37. At 15-year follow-up, Sowers et al. (2010) divided the subjects from SWAN (n=629 women aged 24-44 years at baseline) based on four FSH stages (stage 1=FSH <15, 2=15-33, 3=34-54 and 4≥54 mIU/ml) 38. They observed that annual spinal BMD loss was the highest for those in stage 3 and 4. The BMD for those at stage 4 was 6.4% lower at the spine, and 5% lower at the femoral neck compared to those at stage 1. A higher BMI could attenuate the degree of bone loss 38. The study also showed that the annual bone loss in women two years before menopause was 1.7%, which indicated a significant bone loss even before oestrogen production ceased 38. Therefore, the longitudinal studies validate that premenopausal women with higher FSH level have higher rate of bone loss.

Women Across Menopausal Stages

The relationship between FSH and bone may be dependent on menopausal status. An early study by Ebeling et al. (1996) showed that the negative relationship between FSH and femoral neck and lumbar spine BMD among 281 women aged 45-57 years diminished when menopausal status was adjusted 39. Data from the third US National Health and Nutrition Examination Survey (3247 women aged 42-60 years) showed an inverse association between femoral BMD and FSH among perimenopausal women with high BMI and postmenopausal women with low BMI 40. Elevated FSH level was also associated with increased risk for osteoporosis (odds ratio: 2.59, 95% confidence interval: 1.49-4.49) after adjustment for multiple risk factors 40. There were a number of cross-sectional studies among Asian population pertaining to this issue as well. Yasui et al. (2006) showed that spinal BMD correlated negatively with FSH and positively with oestradiol among 193 Japanese women aged 39-66 years from a university hospital 41. Desai et al. (2007) observed that FSH was the lowest in Indian women (n=365, aged 20-70 years) who belonged to the highest quartiles of lumbar spine and femoral BMD 42. Similarly, Xu et al. (2009) showed that FSH correlated with BMD at spine, total hip and distal forearm in 699 healthy Chinese women aged 20-82 years 43. The prevalence of osteoporosis at 3rd and 4th quartile of FSH was 27.1±8.90% and 30.9±9.89% 43. However, analysis of these three studies lacked proper adjustment for potential confounding factors. The FSH level might be a surrogate for menopausal status in these studies. Wu et al. (2013) estimated the BMD decrease rate among 368 healthy adult Chinese women aged 35-60 years based on the difference between measured BMD of the subjects with the reference peak BMD 44. Lumbar spine and femoral neck BMD correlated negatively with FSH level after adjustment for age and BMI 44. In the multivariate model including FSH, LH and oestradiol, FSH was the most important negative predictors of BMD decrease rate, explaining 18.2%, 33.3% and 29.9% of the variation in the rate at femoral neck, lumbar spine and ultradistal radius and ulna 44. Therefore, it can be concluded that FSH is an important determinant of BMD in women across menopausal stages.

Cross-sectional evaluation of the association between FSH and bone remodelling markers indicated heterogenous results. Ebeling et al. (1996) noted that FSH correlated positively with bone resorption markers (urinary DPD, total PYD, NTX) and bone formation markers (alkaline phosphatase (BAP)) in pre, peri and postmenopausal Australian women 39. Yasui et al. (2006) also showed that FSH correlated positively with intact and uncarboxylated osteocalcin in the Japanese women but they did not adjust for vitamin K status 41. On the other hand, data from Rochester Epidemiology Study involving 188 Caucasian women aged 21-85 years demonstrated that FSH was not associated with any bone remodelling markers (AP, BAP, PYD, DPD) in pre- and postmenopausal women. C-terminal telopeptide was correlated positively with FSH in postmenopausal women before adjustment 45. Instead, inhibin A was the best predictor for bone formation markers and oestradiol was the best predictor for bone resorption markers in these postmenopausal women 45. Despite some inconsistencies, these studies show that high FSH is associated with increased bone remodelling characterized serum/urinary markers.

Crandall et al. (2013) followed a group of pre/perimenopausal women (aged 42-52 years) from SWAN for 10 years and examined their bone changes at before, during and after transmenopausal period 46. During pretransmenopausal period, every doubling of FSH level was associated with a loss of 0.28% in the lumbar spine BMD of the subjects (vs 0.10% slower BMD loss contributed by doubling of oestrogen) 46. In the multivariate model adjusted for oestradiol, testosterone and sex-hormone binding globulin level, only FSH was positively associated with increased lumbar spine BMD loss of -0.32% annually 46. During transmenopausal period, every doubling of FSH was associated with an annual -0.33% BMD change at lumbar spine (vs -0.38% caused by doubling of SHBG) 46. In the adjusted multivariate model, FSH was associated with a reduction of 0.25% BMD annually at femoral neck 46. In late postmenopausal period, lumbar spine BMD loss was associated with oestrogen and SHBG level but not with FSH. No hormone was predictive of femoral neck BMD loss in this period 46. This highlighted the significant role of FSH in bone loss during pre/perimenopausal period, but not postmenopausal when the effects of oestrogen deficiency are prominent.

Postmenopausal women

Several studies scrutinized the skeletal effects of FSH in the postmenopausal population to validate the speculation aforementioned. In 111 community-dwelling multi-ethnic postmenopausal women aged 50-64 years, Gourlay et al. (2011) indicated that both FSH and oestradiol were not significantly associated with BMD at lumbar spine, femoral neck, total hip and distal radius in adjusted multivariate models 47. However, it was a significant negative predictor for trabecular volumetric BMD assessed by pQCT in these women 47. In the subsequent analysis (94 postmenopausal women aged 50-64 years) considering body composition, FSH was significantly and negatively associated with lean mass and bone mass but not BMD 48. Since Bonferroni adjustment, a very conservative approach, was performed in both studies, type II error (false negative) might be inflated. Wang et al. (2015) found a negative correlation between forearm BMD and FSH level in 248 Chinese women aged > 50 years (128 were osteoporotic and 120 had normal bone health) but the analysis was not adjusted for confounding factors 20. The osteoporotic subjects were shown to have a higher FSH and lower oestradiol level in each age group 20. From these studies, it is observed that the relationship between FSH and bone health is between negative to negligible in postmenopausal women. However, causality cannot be inferred because no longitudinal studies on the association between FSH and bone in postmenopausal women have been published.

A gene polymorphism study among 289 postmenopausal women aged 50-75 years showed that BAP and CTX-1 levels were higher, and femoral neck and total body BMD were lower in postmenopausal women with AA (Asn680/Asn680) rs6166 compared with those with GG (Ser680/Ser680) rs6166 FSHR genotype 49. Women with AG (Ser680/Asn680) genotype also showed significantly lower femoral neck and total body BMD and quantitative ultrasound stiffness index compared to those with GG genotype 49. Multiple regression analysis confirmed that women with AA genotype had increased risk for osteoporosis (odds ratio: 1.87, 95% CI: 1.18-2.70) and osteopenia (odds ratio: 1.75, 95% CI: 1.25-2.26) compared to GG genotype after adjustment for various confounding factors. Besides, more subjects with the AA genotype experienced at least one clinical fracture compared to GG genotype 49. This showed that polymorphism of the FSH gene could influence the bone health of women beyond menopausal age.

Men

Osteoporosis is traditionally linked to the gradual decline of testosterone due to age 50, 51. Two independent studies have examined the relationship between FSH and bone in men. In a case control study by Karim et al. (2008) involving 63 community-dwelling osteoporotic and 93 normal men in UK (aged 57.7±13.7 years), FSH was a significant negative predictor of BMD at lumbar spine, femoral neck and hip in an adjusted multivariate model 52. The relationship persisted when case and control were analysed separately 52. Hsu et al. (2015) analysed the data from the Concord Health and Ageing in Men Project, which followed 1705 men aged > 70 years for 5 years 53. The baseline FSH level was negatively associated with BMD change in univariate and multivariate analysis adjusted for age, BMI, smoking status, physical activity and number of comorbidities 53. High FSH was also associated with a higher risk for all types of fracture and hip fracture in univariate model but after adjustment in multivariate model, the association was rendered not significant 53. The authors suggested that since testosterone was not associated with BMD of the subjects, the relationship between bone and FSH could be independent of the androgenic status in these men 53. Despite the limited number of studies compared to women, the current evidence suggests a negative association between bone health and FSH level in men.

Experiment by nature or human

Hyper- and hypogonadotropic conditions induced by diseases and drugs provide an opportunity to study the relationship between FSH and bone in humans. Devleta et al. (2004) studied the spinal and femoral BMD of hypergonadotropic (FSH>40 IU/l; n=7; aged 37.43±3.10 years) and hypogonadotropic (FSH< 40 IU/l; n=15; aged 29.8±5.71 years) amenorrhoeic and eumenorrheic women (n=12; aged 33.81±5.89 years) 54. As expected, the amenorrhoeic women had lower lumbar spine T-score compared to eumenorrheic women 54. Despite the difference in oestradiol level was not statistically significant, hypergonadotropic women were found to have a significant lower lumbar spine BMD than hypogonadotropic women 54. In a group of women aged 45.9±5.5 years diagnosed with breast cancer and receiving cancer chemotherapy for at least one year, FSH was associated with the degree of BMD loss at lumbar spine and femoral neck since treatment initiation 55. The rate of bone loss at lumbar spine was the highest in the highest tertile of FSH 55. In addition, BMD at femoral neck and hip, CTX, PINP and osteocalcin were the lowest in the highest tertile of FSH 55. However, the use of tamoxifen, a known agent that increases BMD, was not adjusted in this study 55. These studies show that alteration of FSH level due to diseases or drugs could also influence bone health in humans.

The bone remodelling markers and BMD of adolescent women with Kallman syndrome (hypogonadotropic; n=8), Turner syndrome (hypergonadotropic; n=11) and pure gonadal dygenesia (hypergonadotropic; n=11) were compared 56. Women with Kallman syndrome had the lowest lumbar spine and hip BMD compared to women with the other two conditions, although the NTX was not significantly different among them 56. There was a significant negative relationship between FSH and spinal BMD in unadjusted correlation test 56. After adjustment for growth hormone therapy, the association was lost 56. In another study, no correlation was found between FSH and total or lumbar spine BMD among 76 long-term survivors treated for paediatric cancer (43 men and 33 women, aged 24.1±3.5 years) 57. Due to the small sample size and heterogeneity of the conditions and treatments in both studies, it is difficult to interpret the relationship between FSH level and bone health in the subjects.

In a clinical trial, post-menopausal women were randomized into leuprolide (7.5 mg i.m. every 28 days; n=21 aged 67.4±1.2 years) and placebo group (n=20 aged 66.1±1.3 years) 58. Both group received letrozole, an aromatase inhibitor to prevent exogenous synthesis of oestradiol 58. At the end of the experiment, both group experienced a significant increase in CTX and TRAP5b level 58. Only the leuprolide group showed increased PINP level 58. Therefore, the inhibition of FSH through leuprolide did not prevent high bone remodelling, but rather enhanced it. Since these women were menopausal, the effects of FSH might be different from women in other stages of life.

The epidemiological studies regarding the relationship between FSH and bone health in humans are summarized in Table 1.

Table 1

The relationship between FSH and bone health in humans.

Authors	Study design	Relationship with variables
		BMD	Bone remodelling markers	pQCT	Fracture
Premenopausal Women
Garton et al. 1996 31	68 spontaneously menstruating women aged 45-55 years. The subjects were divided based on tertiles of FSH level (<10 U/l; 10-35 U/l; >35 U/l).	Negative	Serum phosphate, PYD, DYD: positive
Sowers et al. 2003 33	2336 women aged 42- 52 years (pre and peri menopause) from the Study of Women's Health Across the Nation (SWAN). Composition of the subjects were 28.2% African-American, 49.9% Caucasian, 10.5% Japanese or 11.4% Chinese.	Negative
Sowers et al. 2003 34	2,375 pre- and early perimenopausal women from SWAN, aged 42-52 years. Multiethnicities.		NTX: positiveOsteocalcin: negative
Grewal et al. 2006 35	643 pre- and perimenopausal women, aged 43-53 years from SWAN. BMD at lumbar spine and femoral hip was measured.	Negative
Cannon et al. 2010 32	36 women aged 20-50 years with normal natural menstrual cycles.	Negative
Vural et al. 2005 59	87 healthy volunteers from the community aged 35-50 years.	Not significant	NTX: positive Osteocalcin: not significant
Hui et al. 2002 36	130 non-Hispanic white women aged 31-50 years. Followed up at least 3 times for 1-9 years.	Negative		Negative
Sowers et al. 2006 37	4-year longitudinal study of the SWAN cohort. 2311 premenopausal or early perimenopausal African-American, Caucasian, Chinese, and Japanese women.	Negative
Sowers et al. 2010 38	629 women aged 24 - 44 years at baseline were followed up for 15 years. Subjects were divided into FSH stages 1-4: 1=<15, 2=15-33, 3=34-54, 4=>54 mlU/ml.	Negative
Crandall et al. 2013 46	A 10-year follow up of 720 women in SWAN cohort. Subjects aged 42-52 (mean 46.2) years at baseline.	Negative
Women across menopausal stages
Ebeling et al. 1996 39	281 women aged 45-57 years (pre, peri and postmenopausal groups) selected from a larger randomized urban population cohort (Melbourne Women's Midlife Health Project).	Not significant after adjustment	uDPD, total PYD, NTX, BAP: positive
Perrien et al. 2006 45	188 pre- and postmenopausal women not using oral contraceptives or hormone replacement therapy (age, 21-85 yr) from Rochester Epidemiology Project. Only 2 subjects were non-Caucasians.		CTX: positiveAP, BAP, PYD, DPD: Not significant
Yasui et al. 2006 41	Cross-sectional study. 193 female outpatients of a Japanese university hospital aged 39-66 years. 40 were premenopause, 47 were perimenopause, 106 were postmenopause stage. Serum biochemical markers measured included uncarboxylated osteocalcin, intact osteocalcin, bone alkaline phosphatase, urinary N-telopeptide, LH, FSH, oestradiol, estrone.	Negative	Osteocalcin (intact and uncarboxylated): Positive
Desai et al. 2007 42	365 Indian women aged 20-70 years from a community-based clinic.	Negative
Xu et al. 2009 43	Cross-sectional study. 699 healthy Chinese women aged 20-82 years. Serum LH, FSH measured. BMD measured at posteroanterior spine, lateral spine, TH and distal forearm.	Negative
Gallagher et al. 2010 40	3247 peri- and postmenopausal women aged 42-60 years from US National Health and Nutrition Examination Survey (NHANESIII).	Negative
Wu et al. 2013 44	Cross-sectional study. 368 healthy adult Chinese women (155 premenopausal women, 63 perimenopausal, 150 postmenopausal women), aged 35-60 years.	Negative
Post-menopausal Women
Gourlay et al. 2011 47	111 community-dwelling postmenopausal women aged 50-64 years (mean 57.5 ± 3.7) from various ethnicities.	Negative but lost after adjustment
Gourlay et al. 2012 48	94 younger (aged 50 to 64 years, mean 57.5 years) community dwelling postmenopausal women not using HRT.			Negative
Wang et al. 2015 20	248 postmenopausal Chinese women aged 50 years or above (128 osteoporotic and 120 normal bone health)	Negative
Men
Karim et al. 2008 52	Case-control study. 156 community-dwelling men in London UK aged 57.7 ± 13.7 years. 63 osteoporotic men, 93 normal control.	Negative			Not significant
Hsu et al. 2015 53	1705 men aged 70 years and older from the Concord Health and Ageing in Men Project were followed up for 5 years.	Negative
Experimental by nature or human
Kawai et al. 2004 60	A retrospective study on 125 women undergoing hormone replacement therapy. Sequential measurement of hormone was performed before, at 12 and 24 months after starting hormone replacement therapy.	Negative
Devleta et al. 2004 54	7 hypergonadotropic (FSH>40 IU/l; aged 37.43 ± 3.10), 15 hypogonadotropic (FSH<40 IU/l; aged 29.8 ± 5.71) amenorrhoeic and 12 eumenorrheic women (aged 33.81 ± 5.89) were recruited.	Negative
Castelo-Branco et al. 2008 56	8 adolescent women with Kallman syndrome (hypogonadotropic); 11 with Turner syndrome (hypergonadotropic); 11 with pure gonadal dysgenesia (hypergonadotropic).	Not significant after adjustment
Drake et al. 2010 58	Post-menopausal women were randomized into two groups. One group (n=21, aged 67.4 ± 1.2) received leuprolide (7.5 mg i.m. every 28 d) and the other group (n=20, aged 66.1±1.3 years) received placebo. Both groups received aromatase inhibitor (letrozole, 2.5 mg/d) to prevent exogenous synthesis of oestradiol.		High bone turnover not inhibited.
Latoch et al. 2015 57	76 long-term survivors (43 men and 33 women) treated for paediatric cancer. 38% leukaemia, 36% lymphoma, 26% solid tumours. Age at the study was 24.1 ±3.5 years	Not significant
Tabatabai et al. 2016 55	206 women (64% white) age ≤ 55 (mean 45.9 ±5.5) years at breast cancer diagnosis receiving adjuvant cancer chemotherapy and at least 1 year after diagnosis.	Negative	CTX, PINP, osteocalcin: positiveAP, NTX: Not significant

Abbreviation:

AP=alkaline phosphatase; BAP=bone-specific alkaline phosphatase; BMD=bone mineral density; DPD=deoxypyridinoline; CTX=C-terminal telopeptide of type I collagen; FSH=follicle-stimulating hormone; NTX=N-terminal telopeptide of type I collagen; PINP=N-terminal propeptide of type I procollagen; pQCT=peripheral quantitative computed tomography; PYD=pyridinoline

Conclusion

FSH has a direct effect on bone resorption mediated by FSHR receptors found on osteoclasts and their precursors. The effects of FSH on osteoblasts could be negligible since they do not express FSHR. Transgenic rodent model showed heterogenous results on the skeletal effects of FSH, which seem to be dependent on the ovarian production of testosterone in rodents lacking FSH and FSHR. Supplementing FSH in rats has been shown to be detrimental to the bone, while blocking its activity seems to be beneficial to the skeleton. The human studies generally reveal a significant and negative relationship between FSH level and bone health but the relationship diminishes after menopause, when the effects of oestrogen deficiency are dominant. Thus, FSH may partially explain bone loss during perimenopausal period. Skeletal deterioration in hypogonadotropic hypogonadism may occur because the influence of sex hormone deficiency is greater than FSH deficiency. Similar negative relationship between FSH and bone health is observed in men.

Several research gaps need to be bridged to validate the relationship between FSH and bone health. The current evidence is predominantly from cross-sectional studies which prevents the interpretation of causality. More longitudinal investigations on the effects of FSH on bone health, especially fracture risk in women, should be made. More studies on men should also be performed because their FSH level and fracture risk also increase gradually with age. In addition to that, post-fracture mortality rate of men is higher than women, which necessitates a better understanding of male osteoporosis and its predictors like FSH. Since the hormonal changes across life stages is complex, there is a need to understand the influence of not just FSH alone, but also other related hormone factors, or the whole hormonal milieu alternation on bone health. While the use of anti-FSH antibody to stop bone loss is tempting, there is insufficient evidence currently, to support that blocking the effects of FSH during perimenopause period exerts skeletal beneficial in humans. We hope that more enlightening discoveries in the future will lead to a better understanding of the involvement of FSH in the pathogenesis of osteoporosis in aging women and men. Hopefully, this will spark more innovative and safer interventions to halt bone loss by manipulating the hormonal milieu.