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转化生长因子-β。一种非常有效的成肌细胞分化抑制剂,与水牛大鼠肝细胞分泌的分化抑制剂相同。

Transforming growth factor-beta. A very potent inhibitor of myoblast differentiation, identical to the differentiation inhibitor secreted by Buffalo rat liver cells.

作者信息

Florini J R, Roberts A B, Ewton D Z, Falen S L, Flanders K C, Sporn M B

出版信息

J Biol Chem. 1986 Dec 15;261(35):16509-13.

PMID:3465726
Abstract

Transforming growth factor-beta (TGF-beta) is now known to have a number of actions in addition to the induction of phenotypic transformation in fibroblastic cells. In this paper, we characterize its inhibition of differentiation in rat myoblasts of Yaffe's L6 strain and demonstrate its identity or very close similarity to the differentiation inhibitor (DI) secreted by Buffalo rat liver cells cultured in serum-free medium. At concentrations as low as 60 pg/ml, TGF-beta gave detectable inhibition of differentiation measured as myoblast fusion and creatine kinase elevation; maximal inhibition was observed at and above 0.5 ng/ml (20 pM). The inhibition persisted as long as fresh TGF-beta was added at 48-h intervals, but it was reversed upon removal of the factor. By itself or in the presence of mitogens, TGF-beta had no mitogenic activity in the L6 cells. Concentration dependencies of human TGF-beta and the rat DI were closely parallel in three assays: inhibition of myoblast differentiation, stimulation of normal rat kidney cell growth in soft agar, and competition for displacement of labeled TGF-beta from binding sites on A549 human lung carcinoma cells. We conclude that most if not all of the DI activity found in medium conditioned by Buffalo rat liver cells can be attributed to the presence of TGF-beta or a very similar molecule. These observations also offer a potentially useful approach to study the control of myogenesis; the process(es) can be blocked in cloned L6 myoblasts by incubation with very small quantities of a pure protein in fully defined serum-free medium.

摘要

现在已知转化生长因子-β(TGF-β)除了能诱导成纤维细胞发生表型转化外,还有多种作用。在本文中,我们阐述了它对Yaffe的L6品系大鼠成肌细胞分化的抑制作用,并证明它与在无血清培养基中培养的水牛大鼠肝细胞分泌的分化抑制因子(DI)相同或非常相似。浓度低至60 pg/ml时,TGF-β就能对以成肌细胞融合和肌酸激酶升高来衡量的分化产生可检测到的抑制作用;在0.5 ng/ml(20 pM)及以上时观察到最大抑制作用。只要每隔48小时添加新鲜的TGF-β,这种抑制作用就会持续存在,但去除该因子后抑制作用会逆转。单独或在有丝分裂原存在的情况下,TGF-β在L6细胞中没有促有丝分裂活性。在三种检测中,人TGF-β和大鼠DI的浓度依赖性密切平行:抑制成肌细胞分化、刺激正常大鼠肾细胞在软琼脂中的生长以及竞争从A549人肺癌细胞上的结合位点置换标记的TGF-β。我们得出结论,水牛大鼠肝细胞条件培养基中发现的大部分(如果不是全部)DI活性可归因于TGF-β或非常相似的分子的存在。这些观察结果也为研究肌发生的控制提供了一种潜在有用的方法;通过在完全确定的无血清培养基中与极少量的纯蛋白孵育,该过程可以在克隆的L6成肌细胞中被阻断。

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