TY - JOUR
T1 - Targeted disruption of BMP signaling through type IA receptor (BMPR1A) in osteocyte suppresses SOST and RANKL, leading to dramatic increase in bone mass, bone mineral density and mechanical strength
AU - Kamiya, Nobuhiro
AU - Shuxian, Lin
AU - Yamaguchi, Ryosuke
AU - Phipps, Matthew
AU - Aruwajoye, Olumide
AU - Adapala, Naga Suresh
AU - Yuan, Hui
AU - Kim, Harry K.W.
AU - Feng, Jian Q.
N1 - Funding Information:
This study was supported by an intramural grant from Texas Scottish Rite Hospital for Children (N.K.) and the National Institutes of Health grants DE025014 and R56DE022789 (J.Q. F). We thank Amanda McLerran for animal care and surgical assistance, Reuel Cornelia and Richard Banlaygas for histological preparation, Ito Bone Histomorphometry Institute for measurements, and Ila Oxendine for experiments.
Funding Information:
This work was supported by the Intramural Research Program of Texas Scottish Rite Hospital for Children (N.K.) and the U.S. National Institutes of Health grants DE025014 and R56DE022789 (J.Q.F).
Publisher Copyright:
© 2016 Elsevier Inc.
PY - 2016/10/1
Y1 - 2016/10/1
N2 - Recent studies suggest a critical role of osteocytes in controlling skeletal development and bone remodeling although the molecular mechanism is largely unknown. This study investigated BMP signaling in osteocytes by disrupting Bmpr1a under the Dmp1-promoter. The conditional knockout (cKO) mice displayed a striking osteosclerotic phenotype with increased trabecular bone volume, thickness, number, and mineral density as assessed by X-ray and micro-CT. The bone histomorphometry, H&E, and TRAP staining revealed a dramatic increase in trabecular and cortical bone masses but a sharp reduction in osteoclast number. Moreover, there was an increase in BrdU positive osteocytes (2–5-fold) and osteoid volume (~ 4-fold) but a decrease in the bone formation rate (~ 85%) in the cKO bones, indicating a defective mineralization. The SEM analysis revealed poorly formed osteocytes: a sharp increase in cell numbers, a great reduction in cell dendrites, and a remarkable change in the cell distribution pattern. Molecular studies demonstrated a significant decrease in the Sost mRNA levels in bone (> 95%), and the SOST protein levels in serum (~ 85%) and bone matrices. There was a significant increase in the β-catenin (> 3-fold) mRNA levels as well as its target genes Tcf1 (> 6-fold) and Tcf3 (~ 2-fold) in the cKO bones. We also showed a significant decrease in the RANKL levels of serum proteins (~ 65%) and bone mRNA (~ 57%), and a significant increase in the Opg mRNA levels (> 20-fold) together with a significant reduction in the Rankl/Opg ratio (> 95%), which are responsible for a sharp reduction in the cKO osteoclasts. The values of mechanical strength were higher in cKO femora (i.e. max force, displacement, and work failure). These results suggest that loss of BMP signaling specifically in osteocytes dramatically increases bone mass presumably through simultaneous inhibition of RANKL and SOST, leading to osteoclast inhibition and Wnt activation together. Finally, a working hypothesis is proposed to explain how BMPR1A controls bone remodeling by inhibiting cell proliferation and stimulating differentiation. It is reported that RANKL and SOST are abundantly expressed by osteocytes. Thus, BMP signaling through BMPR1A plays important roles in osteocytes.
AB - Recent studies suggest a critical role of osteocytes in controlling skeletal development and bone remodeling although the molecular mechanism is largely unknown. This study investigated BMP signaling in osteocytes by disrupting Bmpr1a under the Dmp1-promoter. The conditional knockout (cKO) mice displayed a striking osteosclerotic phenotype with increased trabecular bone volume, thickness, number, and mineral density as assessed by X-ray and micro-CT. The bone histomorphometry, H&E, and TRAP staining revealed a dramatic increase in trabecular and cortical bone masses but a sharp reduction in osteoclast number. Moreover, there was an increase in BrdU positive osteocytes (2–5-fold) and osteoid volume (~ 4-fold) but a decrease in the bone formation rate (~ 85%) in the cKO bones, indicating a defective mineralization. The SEM analysis revealed poorly formed osteocytes: a sharp increase in cell numbers, a great reduction in cell dendrites, and a remarkable change in the cell distribution pattern. Molecular studies demonstrated a significant decrease in the Sost mRNA levels in bone (> 95%), and the SOST protein levels in serum (~ 85%) and bone matrices. There was a significant increase in the β-catenin (> 3-fold) mRNA levels as well as its target genes Tcf1 (> 6-fold) and Tcf3 (~ 2-fold) in the cKO bones. We also showed a significant decrease in the RANKL levels of serum proteins (~ 65%) and bone mRNA (~ 57%), and a significant increase in the Opg mRNA levels (> 20-fold) together with a significant reduction in the Rankl/Opg ratio (> 95%), which are responsible for a sharp reduction in the cKO osteoclasts. The values of mechanical strength were higher in cKO femora (i.e. max force, displacement, and work failure). These results suggest that loss of BMP signaling specifically in osteocytes dramatically increases bone mass presumably through simultaneous inhibition of RANKL and SOST, leading to osteoclast inhibition and Wnt activation together. Finally, a working hypothesis is proposed to explain how BMPR1A controls bone remodeling by inhibiting cell proliferation and stimulating differentiation. It is reported that RANKL and SOST are abundantly expressed by osteocytes. Thus, BMP signaling through BMPR1A plays important roles in osteocytes.
UR - http://www.scopus.com/inward/record.url?scp=84978712219&partnerID=8YFLogxK
UR - http://www.scopus.com/inward/citedby.url?scp=84978712219&partnerID=8YFLogxK
U2 - 10.1016/j.bone.2016.07.002
DO - 10.1016/j.bone.2016.07.002
M3 - Article
C2 - 27402532
AN - SCOPUS:84978712219
SN - 8756-3282
VL - 91
SP - 53
EP - 63
JO - Bone
JF - Bone
ER -
