Regulation of human bone marrow-derived osteoprogenitor cells by osteogenic growth factors.

Long, Michael W.; Jeyashakila, Robinson; Ashcraft, E A; Mann, Kenneth G.

doi:10.1172/jci117738

Cited by 216 publications

(156 citation statements)

References 34 publications

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“…Moreover, molecular analysis demonstrated a common retroviral integration site in clonogenic hematopoietic cells and osteoprogenitors from each of seven animals studied, establishing a shared clonal origin for these cell types. These findings thus lent considerable credence to the previous work of Long et al [3,4] and established that, at least in the experimental paradigm used by Dominici and colleagues [9], non-adherent bone marrow cells have a >10-fold more robust bone-repopulating activity than do adherent bone marrow stromal cells. Moreover, the findings were also consistent with previous work by Olmsted-Davis et al [10] suggesting the presence of a unique progenitor cell with both hematopoietic and osteoblastic differentiation potential in the non-adherent subset of bone marrow cells.…”

Section: Introductionsupporting

confidence: 78%

“…We found that OCN pos cells isolated using either the antibody we used in our previous work (SC V-19) [14] or the antibody used by Long and colleagues (HT AON-5031) [3,4] identified very similar populations of cells, at least as assessed by flow cytometry and confocal microscopy. While additional studies need to be done further characterizing the cells isolated with the two antibodies, these data do provide some reassurance that the cells identified in our previous work using the SC V-19 antibody are not some type of spurious population staining only with this particular antibody.…”

Section: Discussionmentioning

confidence: 62%

“…We initially used the anti-OCN antibody utilized in our previous study (SC V-19) [14] and the antibody originally used by Long and colleagues in their work for identifying OCN pos cells in bone marrow (HT AON-5031) [3,4] and verified that both antibodies stained only mineralized matrix and the appropriate cells in normal human bone ( Figure 1A and B). Adjacent muscle or connective tissue of the same section did not stain with the two OCN antibodies ( Figure 1C and D) Human bone incubated just with the secondary antibody served as negative control ( Figure 1E and F).…”

Section: Immunohistochemistry Of Normal Human Bone With Anti-ocn Antimentioning

confidence: 93%

“…Since then, there has been an extensive body of work (summarized in [2]) on the characterization of bone marrow stromal cells with osteoblastic potential in rodent and in human systems. Concurrent with this work, however, Long and colleagues identified, over a decade ago, a non-adherent population of cells in bone marrow with osteogenic potential [3,4]. Rather than selection by adherence to plastic, the primary assay used was cell sorting using antibodies to osteocalcin (OCN), osteonectin, and bone alkaline phosphatase (AP).…”

Section: Introductionmentioning

confidence: 99%

“…Rather than selection by adherence to plastic, the primary assay used was cell sorting using antibodies to osteocalcin (OCN), osteonectin, and bone alkaline phosphatase (AP). When cultured in the presence of TGF-β and accessory bone marrow cells (the identity of which still remains unclear), OCN positive (OCN pos ) cells proliferated and differentiated into mature osteoblastic cells expressing bone-related genes and capable of mineral deposition [3,4]. Somewhat surprisingly, despite the fact that OCN is a secreted protein, these investigators did not need to permeabilize the cells in order to detect cells producing OCN.…”

Section: Introductionmentioning

confidence: 99%

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Characterization of circulating osteoblast lineage cells in humans

Eghbali‐Fatourechi

Mödder

Charatcharoenwitthaya

et al. 2007

Bone

123

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We recently identified circulating osteoblastic cells using antibodies to osteocalcin (OCN) or alkaline phosphatase (AP). We now provide a more detailed characterization of these cells. Specifically, we demonstrate that 46% of OCN positive (OCN pos ) cells express AP, and 37% also express the hematopoietic/endothelial marker, CD34. Using two different anti-OCN antibodies and forward/side light scatter characteristics by flow cytometry, we find that OCN pos cells consist of two distinct populations: one population exhibits low forward/side scatter, consistent with a small cell phenotype with low granularity, and a second population has higher forward/side scatter (larger and more granular cell). The smaller, low granularity population also co-expresses CD34, whereas the larger, more granular cells are CD34 negative. Using samples from 26 male subjects aged 28 to 68 years, we demonstrate that the concentration of circulating OCN pos cells increases as a function of age (R = 0.59, P = 0.002). By contrast, CD34 pos cells tend to decrease with age (R = −0.31, P = 0.18); as a consequence, the ratio of OCN pos :CD34 pos cells also increases significantly with age (R = 0.54, P = 0.022). These findings suggest significant overlap between circulating cells expressing OCN and those expressing the hematopoietic/endothelial marker, CD34. Further studies are needed to define the precise role of circulating OCN pos cells not only in bone remodeling but rather also potentially in the response to vascular injury.

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Section: Introductionsupporting

confidence: 78%

Section: Discussionmentioning

confidence: 62%

Section: Immunohistochemistry Of Normal Human Bone With Anti-ocn Antimentioning

confidence: 93%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 3 more Smart Citations

Characterization of circulating osteoblast lineage cells in humans

Eghbali‐Fatourechi

Mödder

Charatcharoenwitthaya

et al. 2007

Bone

123

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Prostaglandin E1 and recombinant bone morphogenetic protein effect on strength of hydroxyapatite implants

Ono

Tateshita

Kuboki

1999

J. Biomed. Mater. Res.

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Although combinations of hydroxyapatite (HAP) and bone morphogenetic protein (BMP) are expected to provide potent alternatives to autogenous bone grafts, it is still anticipated that substances that act synergistically with BMP will be found because the inducing potential of purified BMP in bone is not strong enough. We already have shown that prostaglandin (PG) E1 has a strong and dose-dependent synergistic effect on the osteoinductive activity induced by recombinant human (rh) BMP and that it enhances osteoconduction even when used alone. In this study, porous HAP rods were treated as follows: (1) without PGE1 or rhBMP (control group); (2) with varying concentrations of PGE1; and (3) with varying concentrations of PGE1 combined with 1 microg of rhBMP-2. The rods were subperiosteally implanted on the cranial bone of rabbits to evaluate the effect of these treatments on the mechanical strength of the implanted HAP rods. The HAP rods were removed 3, 6, or 9 weeks after implantation and subjected to mechanical strength determinations. The control group (no addition of BMP to the rods) showed no significant increase in three-point bending strength or in compression strength compared to pre-implantation. On the other hand, PGE1 combined with rhBMP had a strong and dose-dependent effect on the mechanical strength of HAP, increasing it significantly, especially compression strength. PGE1 also increased mechanical strength even when used alone. Histological examination revealed that PGE1, whether or not it was combined with rhBMP, increased bone formation into the pores of HAP and consequently increased the mechanical strength of porous HAP.

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Regulation of bone matrix protein expression and induction of differentiation of human osteoblasts and human bone marrow stromal cells by bone morphogenetic protein-2

1997

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We have examined the effects of BMP-2 on the expression of bone matrix proteins in both human bone marrow stromal cells (HBMSC) and human osteoblasts (HOB) and their proliferation and mineralization. Both HBMSC and HOB express BMP-2/-4 type I and type II receptors. Treatment of these two cell types with BMP-2 for 4 weeks in the presence of beta-glycerophosphate and ascorbic acid results in mineralization of their matrix. BMP-2 increases the mRNA level and activities of alkaline phosphatase and elevates the mRNA levels and protein synthesis of osteopontin, bone sialoprotein, osteocalcin, and alpha 1(I) collagen in both cell types. Whereas the mRNA level of decorin is increased, the mRNA concentration of biglycan is not altered by BMP-2. No effect on osteonectin is observed. The effect of BMP-2 on bone matrix protein expression is dose dependent from 25 to 100 ng/ml and is evident after 1-7 days treatment. In the presence of BMP-2, proliferation of HBMSC and HOB is decreased under either serum-free condition or in the presence of serum. Thus, BMP-2 has profound effects on the proliferation, expression of most of the bone matrix proteins and the mineralization of both relatively immature human bone marrow stromal preosteoblasts and mature human osteoblasts.

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Regulation of human bone marrow-derived osteoprogenitor cells by osteogenic growth factors.

Cited by 216 publications

References 34 publications

Characterization of circulating osteoblast lineage cells in humans

Characterization of circulating osteoblast lineage cells in humans

Prostaglandin E1 and recombinant bone morphogenetic protein effect on strength of hydroxyapatite implants

Regulation of bone matrix protein expression and induction of differentiation of human osteoblasts and human bone marrow stromal cells by bone morphogenetic protein-2

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