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首页> 外文期刊>Journal of bone and mineral research: the official journal of the American Society for Bone and Mineral Research >Chinese hamster ovary cells expressing alpha4beta1 integrin stimulate osteoclast formation in vitro.
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Chinese hamster ovary cells expressing alpha4beta1 integrin stimulate osteoclast formation in vitro.

机译:表达α4β1整合素的中国仓鼠卵巢细胞在体外刺激破骨细胞形成。

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摘要

It is reported that Chinese hamster ovary cells transfected with human alpha4 cDNA (alpha4CHOs) and expressing functional alpha4beta1 integrin developed bone metasasis in nude mice. To clarify the role of alpha4beta1 integrin in bone metastasis, in terms of tumor-mediated bone destruction, we examined whether alpha4CHOs stimulate osteoclast formation in cocultures with mouse bone marrow cells. The number of osteoclast-like cells identified as tartrate-resistant acid phosphatase positive multinucleated cells (TRAP(+) MNCs) formed from bone marrow cells increased with the increasing number of alpha4CHOs cocultured. The effects of 1,25-dihydroxyvitamin D3 (1,25(OH)2D3) and prostaglandin E2 (PGE2) on TRAP(+) MNC formation were enhanced in cocultures with alpha4CHOs. TRAP(+) MNCs induced by alpha4CHOs possessed calcitonin receptors and resorbed calcified tissues. In cocultures, alpha4CHOs and bone marrow stromal cells were in contact with each other and bone marrow stromal cells expressed vascular cell adhesion molecule-1 (VCAM-1), which is one of the ligands for alpha4beta1 integrin. TRAP(+) MNC formation was not stimulated in cocultures where direct contact between alpha4CHOs and bone marrow cells was inhibited by membrane filters. Alpha4CHOs do not support TRAP(+) MNC formation in cocultures with spleen cells but do support TRAP(+) mononuclear cell and MNC formation from spleen cells in the presence of osteoblastic cells. Cultured media from alpha4CHOs, bone marrow cells, and cocultures of alpha4CHOs and bone marrow cells did not stimulate TRAP(+) MNC formation or enhance the effects of 1,25(OH)2D3 and PGE2 in bone marrow cultures. The concentrations of PGE2 and interleukin-6 (IL-6) in cultured media were not different between the cultures of bone marrow cells and the cocultures of bone marrow cells and alpha4CHOs. Anti-human alpha4 and anti-mouse VCAM-1 antibodies inhibited TRAP(+) MNC formation induced by alpha4CHOs. These results indicate that alpha4CHOs stimulated TRAP(+) MNC formation through direct cell-to-cell interaction between alpha4beta1 and VCAM-1. It is suggested that in addition to various soluble factors regulating osteoclast formation, cell-to-cell interaction between tumor cells and bone marrow cells is important for inducing osteoclasts at the site of bone metastasis and leading to bone destruction.
机译:据报道,用人α4cDNA(α4CHOs)转染并表达功能性α4beta1整合素的中国仓鼠卵巢细胞在裸鼠体内发生骨转移。为了阐明α4beta1整合素在骨转移中的作用,就肿瘤介导的骨破坏而言,我们检查了α4CHOs是否在与小鼠骨髓细胞共培养物中刺激破骨细胞形成。由骨髓细胞形成的抗酒石酸酸性磷酸酶阳性多核细胞(TRAP(+)MNCs)的破骨细胞样细胞的数量随着共培养的alpha4CHOs数量的增加而增加。 1,25-二羟基维生素D3(1,25(OH)2D3)和前列腺素E2(PGE2)对TRAP(+)MNC形成的影响在与alpha4CHOs的共培养中得到增强。由alpha4CHOs诱导的TRAP(+)MNC具有降钙素受体和吸收的钙化组织。在共培养中,alpha4CHOs与骨髓基质细胞相互接触,并且骨髓基质细胞表达了血管细胞粘附分子1(VCAM-1),这是alpha4beta1整联蛋白的配体之一。共培养中未刺激TRAP(+)MNC的形成,其中膜过滤器抑制了alpha4CHOs与骨髓细胞之间的直接接触。 Alpha4CHOs在与脾细胞共培养时不支持TRAP(+)MNC的形成,但是在成骨细胞存在的情况下,它支持TRAP(+)单核细胞和由脾细胞形成的MNC。来自alpha4CHOs,骨髓细胞以及alpha4CHOs与骨髓细胞的共培养物的培养基不会刺激TRAP(+)MNC的形成,也不会增强1,25(OH)2D3和PGE2在骨髓培养物中的作用。骨髓细胞培养物与骨髓细胞和α4CHOs共培养物之间培养基中PGE2和白介素6(IL-6)的浓度没有差异。抗人alpha4和抗小鼠VCAM-1抗体抑制由alpha4CHOs诱导的TRAP(+)MNC形成。这些结果表明alpha4CHOs通过alpha4beta1和VCAM-1之间的直接细胞间相互作用刺激了TRAP(+)MNC的形成。提示除了调节破骨细胞形成的各种可溶性因子外,肿瘤细胞与骨髓细胞之间的细胞间相互作用对于在骨转移部位诱导破骨细胞并导致骨破坏也很重要。

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