Bone marrow stroma in humans: anti-nerve growth factor receptor antibodies selectively stain reticular cells in vivo and in vitro

Cattoretti, Giorgio; Schirò, R; Orazi, Attilio; Soligo, Davide; Colombo, Mario P.

doi:10.1182/blood.v81.7.1726.1726

Cited by 142 publications

(59 citation statements)

References 48 publications

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“…Our findings corroborate previous reports demonstrating that BMSCs isolated from healthy donors express BDNF high affinity receptor TrkB, indicating that paracrine BDNF signaling in the marrow microenvironment may occur. ( 16–18 ) The data suggested that the addition of BDNF can stimulate VEGF secretion by BMSC, and this effect can be blocked by K252α, which is an specific inhibitor of TrkB. We further detected VEGF secretion by MM cell lines and BMSCs isolated from healthy donors.…”

Section: Discussionmentioning

confidence: 85%

“…Besides its frequent expression by malignant plasma cells, TrkB was found to be expressed by osteoblasts, endothelial cells, and BMSCs in the BM microenvironment. ( 16–18 ) Since BDNF and its receptor TrkB expressed by MM cells contribute to plasma cell survival, TrkB expressed by BMSCs may allow stroma–myeloma cell interaction, further influencing BM angiogenesis via secreting angiogenic cytokines. In addition, studies of our group found that the increased serum BDNF levels detected in patients with MM correlated with disease activity and serum VEGF levels.…”

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confidence: 99%

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Lentiviral shRNA silencing of BDNF inhibits in vivo multiple myeloma growth and angiogenesis via down‐regulated stroma‐derived VEGF expression in the bone marrow milieu

Zhang

Sun

et al. 2010

Cancer Science

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Bone marrow (BM) neovascularization and vascular endothelial growth factor (VEGF) expression in multiple myeloma (MM) correlate with disease progression. Brain derived neurotrophic factor (BDNF) is highly expressed by malignant plasma cells isolated from the majority of MM patients. Recently, BDNF was identified as a potential proangiogenic factor for the promotion of endothelial cell survival, induction of neoangiogenesis in ischemic tissues, and increase of VEGF expression in neuroblastoma. Since tropomyosin receptor kinase B (TrkB), the receptor of BDNF, is expressed by stromal cells within the BM milieu, here we sought to evaluate the involvement of BDNF/TrkB in myeloma–marrow stroma interaction and its effects on BM angiogenesis. TrkB was abundantly expressed by bone marrow stromal cells (BMSCs) isolated from healthy donors. Stimulation of BMSCs with BDNF induced a time‐ and dose‐ dependent increase in VEGF secretion, which was completely abolished by K252α, an inhibitor of TrkB. BDNF triggered activation of signal transducer and activator of transcription 3 (STAT3) and activator protein‐1 (AP‐1), whereas STAT3 was involved in mediating VEGF expression. We further delineated the biological significance of BDNF in MM by using lentiviral short‐interfering RNA (shRNA). When myeloma cells were cocultured with BMSCs in a noncontact Transwell system, VEGF levels in supernatants were significantly decreased when BDNF expression was knocked down. Furthermore, silencing of BDNF expression significantly inhibited xenograft tumor growth and angiogenesis, and prolonged survival in mouse model. Our studies demonstrate that BDNF, as a potential stimulator of angiogenesis, contributes to MM tumorgenesis; it mediates stromal–MM cell interactions via selective activation of specific receptor TrkB and downstream signal transducer STAT3, regulating VEGF secretion. (Cancer Sci 2010; 101: 1117–1124)

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Section: Discussionmentioning

confidence: 85%

mentioning

confidence: 99%

Lentiviral shRNA silencing of BDNF inhibits in vivo multiple myeloma growth and angiogenesis via down‐regulated stroma‐derived VEGF expression in the bone marrow milieu

Zhang

Sun

et al. 2010

Cancer Science

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“…The bone marrow stromal microenvironment is composed of cells, structural fibrils and extracellular matrix (‘ground substance’). The cellular components include macrophages, fibroblastic cells (including several types of adventitial and reticular cells), adipocytes and endothelial cells, as well as other less well characterized cells (Weiss & Chen, 1975; Watanabe, 1985; Cattoretti et al , 1993). The most common structural fibrils in the bone marrow are collagen, reticulin, laminin and fibronectin (Bentley et al , 1981; Reilly et al , 1985; Cattoretti et al , 1993).…”

Section: Bone Marrow Microenvironmentmentioning

confidence: 99%

Bone marrow fibrosis: pathophysiology and clinical significance of increased bone marrow stromal fibres

et al. 2007

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SummaryIn bone marrow biopsies, stromal structural fibres are detected by reticulin and trichrome stains, routine stains performed on bone marrow biopsy specimens in diagnostic laboratories. Increased reticulin staining (reticulin fibrosis) is associated with many benign and malignant conditions while increased trichrome staining (collagen fibrosis) is particularly prominent in late stages of severe myeloproliferative diseases or following tumour metastasis to the bone marrow. Recent evidence has shown that the amount of bone marrow reticulin staining often exhibits no correlation to disease severity, while the presence of type 1 collagen, as detected by trichrome staining, is often associated with more severe disease and a poorer prognosis. It was originally thought that increases in bone marrow stromal fibres themselves contributed to the haematopoietic abnormalities seen in certain diseases, but recent studies suggest that these increases are a result of underlying cellular abnormalities rather than a cause. A growing body of evidence suggests that increased deposition of bone marrow stromal fibres is mediated by transforming growth factor-b and other factors elaborated by megakaryocytes, but it is likely that other cells, cytokines and growth factors are also involved. This suggests new avenues for investigation into the pathogenesis of various disorders associated with increased bone marrow stromal fibres.

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“…Although CD15, CD33, CD34, and CD13 are known to be the most common antigens expressed in M1 patients (Foon and Todd, 1986), there are reports describing the expression of CD13 on various non‐hematopoietic cells, including epithelial cells from renal proximal tubules and intestinal brush border, endothelial cells, fibroblasts, brain cells, and bone MSC (Look et al, 1986). Furthermore, detailed immuno‐EM characterization of human bone MSC revealed the expression of CD13 as well as the nerve growth factor receptor (NGFR), alkaline phosphatase, reticulin, collagen III, and vimentin (Cattoretti et al, 1993). In this study, the high expression of CD13 in AML‐I cells does not exclude the possibility of a myeloid cell origin for AML‐I cells, but a defect in the expression of other leukemia‐associated antigens strongly support the idea of a mesenchymal origin for AML‐I cells rather than a hematopoietic origin.…”

Section: Discussionmentioning

confidence: 99%

Establishment of a human preadipose cell line, HPB‐AML‐I: Refractory to PPARγ‐mediated adipogenic stimulation

Torii

Morikawa

Nakano

et al. 2003

Journal Cellular Physiology

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In this study, we established a unique cell line, HPB-AML-I (AML-I), from peripheral blood mononuclear cells collected from a patient with acute myeloid leukemia (AML: M1). Morphological and phenotypical analyses of the established AML-I cells demonstrated that they belong to a preadipocyte cell line as indicated by their storage of lipid droplets and expression of surface antigens similar to those found on bone marrow stromal cells (MSC). Through cell culture under adipogenic conditions, effective differentiation of AML-I cells into adipocytes was induced by an adipogenesis inducing cocktail (INC) made up of a mixture of methylisobutylxanthine, hydrocortisone, and indomethacin. By contrast, activation of peroxisome proliferator-activated receptor (PPARgamma), which plays a key role in lipids metabolism and is highly expressed in AML-I cells, decreased the number of lipid droplets in AML-I cells. Here we report the establishment of a unique human derived-preadipocyte cell line, AML-I, and its bi-directional adipogenic response to different type stimulation, i.e., one is a refractory response to troglitazone, a well-known adipogenic stimulator, and a positive response to INC, an adipogenesis induction cocktail. These results suggest that, based on the adipogenic response, there might be some distinct lineages in human adipocytes and that the unique differentiation of AML-I cells should be useful for analyzing both the differentiation and regulation of human preadipocytes.

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Bone marrow stroma in humans: anti-nerve growth factor receptor antibodies selectively stain reticular cells in vivo and in vitro

Cited by 142 publications

References 48 publications

Lentiviral shRNA silencing of BDNF inhibits in vivo multiple myeloma growth and angiogenesis via down‐regulated stroma‐derived VEGF expression in the bone marrow milieu

Lentiviral shRNA silencing of BDNF inhibits in vivo multiple myeloma growth and angiogenesis via down‐regulated stroma‐derived VEGF expression in the bone marrow milieu

Bone marrow fibrosis: pathophysiology and clinical significance of increased bone marrow stromal fibres

Establishment of a human preadipose cell line, HPB‐AML‐I: Refractory to PPARγ‐mediated adipogenic stimulation

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