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鸡生长板软骨细胞在短期单层培养中转化生长因子-β的产生

The production of transforming growth factor-beta by chick growth plate chondrocytes in short term monolayer culture.

作者信息

Gelb D E, Rosier R N, Puzas J E

机构信息

Department of Orthopedics, University of Rochester Medical Center, New York 14642.

出版信息

Endocrinology. 1990 Oct;127(4):1941-7. doi: 10.1210/endo-127-4-1941.

DOI:10.1210/endo-127-4-1941
PMID:2401238
Abstract

Transforming growth factor-beta (TGF beta) is capable of regulating the proliferation and phenotypic expression of growth plate chondrocytes in culture. Chondrocytes were isolated from the growth plates from the long bones of 3- to 5-week-old chicks. Conditioned medium was harvested from short term monolayer cultures for the assay of TGF beta production by these cells. A receptor competition assay using [125I]TGF beta was used to quantitate the amount of TGF beta in the conditioned medium. Acid-activated conditioned medium contained 5.0 +/- 0.4 ng/ml TGF beta, while conditioned medium that had not been exposed to acid had undetectable levels of the peptide by this assay. The initial cell plating density was inversely related to the amount of TGF beta produced on a per cell basis. Growth plate chondrocytes separated by countercurrent centrifugal elutriation into maturationally distinct subpopulations had different rates of TGF beta production; hypertropic chondrocytes produced significantly more TGF beta (4.5 ng/10(6) cells) than the smallest chondrocytes isolated (2.3 ng/10(6) cells). A variety of other growth mediators were tested for their ability to influence TGF beta production by chondrocytes, and it was found that only basic fibroblast growth factor could significantly influence TGF beta production, producing a 6-fold increase in TGF beta recovered in the conditioned medium. The production of TGF beta by growth plate chondrocytes implicates it as an important autocrine or paracrine regulator in the process of endochondral calcification.

摘要

转化生长因子-β(TGF-β)能够调节培养的生长板软骨细胞的增殖和表型表达。从3至5周龄雏鸡的长骨生长板中分离软骨细胞。从短期单层培养物中收获条件培养基,用于检测这些细胞产生的TGF-β。使用[125I]TGF-β的受体竞争测定法来定量条件培养基中TGF-β的量。酸激活的条件培养基含有5.0±0.4 ng/ml的TGF-β,而未暴露于酸的条件培养基通过该测定法检测不到该肽的水平。初始细胞接种密度与每个细胞产生的TGF-β量呈负相关。通过逆流离心淘析分离成成熟不同亚群的生长板软骨细胞具有不同的TGF-β产生速率;肥大软骨细胞产生的TGF-β(4.5 ng/10(6)个细胞)比分离出的最小软骨细胞(2.3 ng/10(6)个细胞)明显更多。测试了多种其他生长介质影响软骨细胞产生TGF-β的能力,发现只有碱性成纤维细胞生长因子能显著影响TGF-β的产生,使条件培养基中回收的TGF-β增加6倍。生长板软骨细胞产生TGF-β表明它在软骨内钙化过程中是一种重要的自分泌或旁分泌调节因子。

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