Targeted Overexpression of Insulin-Like Growth Factor I to Osteoblasts of Transgenic Mice: Increased Trabecular Bone Volume without Increased Osteoblast Proliferation<sup>1</sup>

Guisheng Zhao(University of Cincinnati Medical Center), Marie-Claude Monier-Faugere(University of Kentucky), M. Chris Langub(University of Kentucky), Zhaopo Geng(University of Kentucky), Toshiyuki Nakayama(University of Cincinnati Medical Center), J. Wesley Pike(University of Cincinnati Medical Center), Steven D. Chernausek(Boston Children's Hospital), Clifford J. Rosen(St. Joseph Hospital), Leah‐Rae Donahue(St. Joseph Hospital), Hartmut H. Malluche(University of Kentucky), James A. Fagin(University of Cincinnati Medical Center), Thomas L. Clemens(United States Department of Veterans Affairs)
Endocrinology
July 1, 2000
Cited by 359Open Access
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Abstract

Insulin-like growth factor I (IGF-I) is an important growth factor for bone, yet the mechanisms that mediate its anabolic activity in the skeleton are poorly understood. To examine the effects of locally produced IGF-I in bone in vivo, we targeted expression IGF-I to osteoblasts of transgenic mice using a human osteocalcin promoter. The IGF-I transgene was expressed in bone osteoblasts in OC-IGF-I transgenic mice at high levels in the absence of any change in serum IGF-I levels, or of total body growth. Bone formation rate at the distal femur in 3-week-old OC-IGF-I transgenic mice was approximately twice that of controls. By 6 weeks, bone mineral density as measured by dual energy x-ray, and quantitative computed tomography was significantly greater in OC-IGF-I transgenic mice compared with controls. Histomorphometric measurements revealed a marked (30%) increase femoral cancellous bone volume in the OC-IGF-I transgenic mice, but no change in the total number of osteoblasts or osteoclasts. Transgenic mice also demonstrated an increase in the osteocyte lacunea occupancy, suggesting that IGF-I may extend the osteocyte life span. We conclude that IGF-I produced locally in bone osteoblasts exerts its anabolic effect primarily by increasing the activity of resident osteoblasts.


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