Your search keyword '"Ominsky, Michael S"' showing total 3 results

1. Sclerostin antibody administration converts bone lining cells into active osteoblasts

Author

Kim, Sang Wan, Lu, Yanhui, Williams, Elizabeth A., Lai, Forest, Lee, Ji Yeon, Enishi, Tetsuya, Balani, Deepak H., Ominsky, Michael S., Ke, Hua Zhu, Kronenberg, Henry M., and Wein, Marc N.

Subjects

Adipogenesis, Osteoblasts, fungi, Adipocytes, Osteocytes, Article

Abstract

Sclerostin antibody (Scl-Ab) increases osteoblast activity, in part through increasing modeling-based bone formation on previously quiescent surfaces. Histomorphometric studies have suggested that this might occur through conversion of bone lining cells into active osteoblasts. However, direct data demonstrating Scl-Ab-induced conversion of lining cells into active osteoblasts is lacking. Here, we used in vivo lineage tracing to determine if Scl-Ab promotes the conversion of lining cells into osteoblasts on periosteal and endocortical bone surfaces in mice. Two independent, tamoxifen-inducible lineage tracing strategies were used to label mature osteoblasts and their progeny using the DMP1 and osteocalcin promoters. Following a prolonged ‘chase’ period, the majority of labeled cells on bone surfaces assumed a thin, quiescent morphology. Then, mice were treated with either vehicle or Scl-Ab (25 mg/kg) twice over the course of the subsequent week. After sacrifice, marked cells were enumerated, their thickness quantified, and proliferation and apoptosis examined. Scl-Ab led to a significant increase in the average thickness of labeled cells on periosteal and endocortical bone surfaces, consistent with osteoblast activation. Scl-Ab did not induce proliferation of labeled cells, and Scl-Ab did not regulate apoptosis of labeled cells. Therefore, direct reactivation of quiescent bone lining cells contributes to the acute increase in osteoblast numbers following Scl-Ab treatment in mice.

Published

2017

2. Sclerostin antibody treatment improves the bone phenotype of Crtap−/− mice, a model of recessive Osteogenesis Imperfecta

Author

Grafe, Ingo, Alexander, Stefanie, Yang, Tao, Lietman, Caressa, Homan, Erica P, Munivez, Elda, Chen, Yuqing, Jiang, Ming Ming, Bertin, Terry, Dawson, Brian, Asuncion, Franklin, Ke, Hua Zhu, Ominsky, Michael S, and Lee, Brendan

Subjects

Mice, Knockout, Extracellular Matrix Proteins, Osteoclasts, Proteins, Genes, Recessive, Osteogenesis Imperfecta, Article, Antibodies, Mice, Osteogenesis, Animals, Intercellular Signaling Peptides and Proteins, Adaptor Proteins, Signal Transducing, Glycoproteins, Molecular Chaperones

Abstract

Osteogenesis imperfecta (OI) is characterized by low bone mass, poor bone quality, and fractures. Standard treatment for OI patients is limited to bisphosphonates, which only incompletely correct the bone phenotype, and seem to be less effective in adults. Sclerostin-neutralizing antibodies (Scl-Ab) have been shown to be beneficial in animal models of osteoporosis, and dominant OI resulting from mutations in the genes encoding type I collagen. However, Scl-Ab treatment has not been studied in models of recessive OI. Cartilage-associated protein (CRTAP) is involved in posttranslational type I collagen modification, and its loss of function results in recessive OI. In this study, we treated 1-week-old and 6-week-old Crtap(-/-) mice with Scl-Ab for 6 weeks (25 mg/kg, s.c., twice per week), to determine the effects on the bone phenotype in models of "pediatric" and "young adult" recessive OI. Vehicle-treated Crtap(-/-) and wild-type (WT) mice served as controls. Compared with control Crtap(-/-) mice, micro-computed tomography (μCT) analyses showed significant increases in bone volume and improved trabecular microarchitecture in Scl-Ab-treated Crtap(-/-) mice in both age cohorts, in both vertebrae and femurs. Additionally, Scl-Ab improved femoral cortical parameters in both age cohorts. Biomechanical testing showed that Scl-Ab improved parameters of whole-bone strength in Crtap(-/-) mice, with more robust effects in the week 6 to 12 cohort, but did not affect the increased bone brittleness. Additionally, Scl-Ab normalized the increased osteoclast numbers, stimulated bone formation rate (week 6 to 12 cohort only), but did not affect osteocyte density. Overall, our findings suggest that Scl-Ab treatment may be beneficial in the treatment of recessive OI caused by defects in collagen posttranslational modification. © 2015 American Society for Bone and Mineral Research.

Published

2016

3. Are osteoclasts needed for the bone anabolic response to parathyroid hormone? A study of intermittent parathyroid hormone with denosumab or alendronate in knock-in mice expressing humanized RANKL

Author

Pierroz, Dominique D., Bonnet, Nicolas, Baldock, Paul A., Ominsky, Michael S., Stolina, Marina, Kostenuik, Paul J., and Ferrari, Serge L.

Subjects

musculoskeletal diseases, Male, Biological Markers/metabolism, Ovariectomy, Osteoclasts, Gene Expression, Parathyroid Hormone/administration & dosage/*pharmacology, Antibodies, Monoclonal, Humanized, Bone and Bones, Antibodies, Monoclonal/administration & dosage/*pharmacology, Mice, Bone Density, Osteogenesis, Alendronate/administration & dosage/*pharmacology, Animals, Humans, RANK Ligand/administration & dosage/*pharmacology, Gene Knock-In Techniques, Bone Resorption, Alendronate, Receptor Activator of Nuclear Factor-kappa B, Dose-Response Relationship, Drug, RANK Ligand, Antibodies, Monoclonal, Bone Density/drug effects, Bone Resorption/drug therapy, Bone and Bones/cytology/drug effects/*metabolism/physiology, Osteogenesis/drug effects, Metabolism, Parathyroid Hormone, ddc:618.97, Female, Osteoclasts/*drug effects/metabolism, Denosumab, Biomarkers, Receptor Activator of Nuclear Factor-kappa B/antagonists & inhibitors/deficiency/*genetics/metabolism

Abstract

PTH stimulates osteoblastic cells to form new bone and to produce osteoblast-osteoclast coupling factors such as RANKL. Whether osteoclasts or their activity are needed for PTH anabolism remains uncertain. We treated ovariectomized huRANKL knock-in mice with a human RANKL inhibitor denosumab (DMAb), alendronate (Aln), or vehicle for 4 weeks, followed by co-treatment with intermittent PTH for 4 weeks. Loss of bone mass and microarchitecture was prevented by Aln and further significantly improved by DMAb. PTH improved bone mass, microstructure, and strength, and was additive to Aln but not to DMAb. Aln inhibited biochemical and histomorphometrical indices of bone turnover,--i.e. osteocalcin and bone formation rate (BFR) on cancellous bone surfaces-, and Dmab inhibited them further. However Aln increased whereas Dmab suppressed osteoclast number and surfaces. PTH significantly increased osteocalcin and bone formation indices, in the absence or presence of either antiresorptive, although BFR remained lower in presence of Dmab. To further evaluate PTH effects in the complete absence of osteoclasts, high dose PTH was administered to RANK(-/-) mice. PTH increased osteocalcin similarly in RANK(-/-) and WT mice. It also increased BMD in RANK(-/-) mice, although less than in WT. These results further indicate that osteoclasts are not strictly required for PTH anabolism, which presumably still occurs via stimulation of modeling-based bone formation. However the magnitude of PTH anabolic effects on the skeleton, in particular its additive effects with antiresorptives, depends on the extent of the remodeling space, as determined by the number and activity of osteoclasts on bone surfaces.

Published

2010