Literature DB >> 11393789

Number and proliferative capacity of osteogenic stem cells are maintained during aging and in patients with osteoporosis.

K Stenderup1, J Justesen, E F Eriksen, S I Rattan, M Kassem.   

Abstract

Decreased bone formation is an important pathophysiological mechanism responsible for bone loss associated with aging and osteoporosis. Osteoblasts (OBs), originate from mesenchymal stem cells (MSCs) that are present in the bone marrow and form colonies (termed colony-forming units-fibroblastic [CFU-Fs]) when cultured in vitro. To examine the effect of aging and osteoporosis on the MSC population, we quantified the number of MSCs and their proliferative capacity in vitro. Fifty-one individuals were studied: 38 normal volunteers (23 young individuals [age, 22-44 years] and 15 old individuals [age, 66-74 years]) and 13 patients with osteoporosis (age, 58-83 years). Bone marrow was aspirated from iliac crest; mononuclear cells were enriched in MSCs by magnetic activated cell sorting (MACS) using STRO-1 antibody. Total CFU-F number, size distribution, cell density per CFU-F, number of alkaline phosphatase positive (ALP+) CFU-Fs, and the total ALP+ cells were determined. In addition, matrix mineralization as estimated by alizarin red S (AR-S) staining was quantified. No significant difference in colony-forming efficiency between young individuals (mean +/- SEM; 87 +/- 12 CFU-Fs/culture), old individuals (99 +/- 19 CFU-Fs/culture), and patients with osteoporosis (129 +/- 13 CFU-Fs/culture; p = 0.20) was found. Average CFU-F size and cell density per colony were similar in the three groups. Neither the percentage of ALP+ CFU-Fs (66 +/- 6%, 65 +/- 7%, and 72 +/- 4% for young individuals, old individuals, and patients with osteoporosis, respectively) nor the percentage of ALP+ cells per culture (34 +/- 5%, 40 +/- 6%, and 41 +/- 4%) differed between groups. Finally, mineralized matrix formation was similar in young individuals, old individuals, and patients with osteoporosis. Our study shows that the number and proliferative capacity of osteoprogenitor cells are maintained during aging and in patients with osteoporosis and that other mechanisms must be responsible for the defective osteoblast (OB) functions observed in these conditions.

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Year:  2001        PMID: 11393789     DOI: 10.1359/jbmr.2001.16.6.1120

Source DB:  PubMed          Journal:  J Bone Miner Res        ISSN: 0884-0431            Impact factor:   6.741


  56 in total

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Review 2.  Angiogenesis and marrow stromal cell fates: roles in bone strength.

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4.  Heparan sulfate enhances the self-renewal and therapeutic potential of mesenchymal stem cells from human adult bone marrow.

Authors:  Torben Helledie; Christian Dombrowski; Bina Rai; Zophia X H Lim; Ian Lee Hock Hin; David A Rider; Gary S Stein; Wanjin Hong; Andre J van Wijnen; James H Hui; Victor Nurcombe; Simon M Cool
Journal:  Stem Cells Dev       Date:  2012-01-18       Impact factor: 3.272

Review 5.  Mesenchymal stem cells: lineage, plasticity, and skeletal therapeutic potential.

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Review 6.  Plasticity of epidermal stem cells: survival in various environments.

Authors:  Jackie R Bickenbach; Matthew M Stern
Journal:  Stem Cell Rev       Date:  2005       Impact factor: 5.739

7.  Osteogenic abilities of bone marrow stromal cells are not defective in patients with osteonecrosis.

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8.  Comparison of potentials of stem cells isolated from tendon and bone marrow for musculoskeletal tissue engineering.

Authors:  Qi Tan; Pauline Po Yee Lui; Yun Feng Rui; Yin Mei Wong
Journal:  Tissue Eng Part A       Date:  2011-12-13       Impact factor: 3.845

9.  Phenotypic Characterization of Mesenchymal Stem Cells from Various Tissues.

Authors:  Markus Thomas Rojewski; Barbara Maria Weber; Hubert Schrezenmeier
Journal:  Transfus Med Hemother       Date:  2008-05-16       Impact factor: 3.747

Review 10.  Mesodermal fate decisions of a stem cell: the Wnt switch.

Authors:  L A Davis; N I Zur Nieden
Journal:  Cell Mol Life Sci       Date:  2008-09       Impact factor: 9.261

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