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转化生长因子-β1对成骨细胞MC3T3-E1中赖氨酰氧化酶的翻译前和翻译后调控

Pre- and post-translational regulation of lysyl oxidase by transforming growth factor-beta 1 in osteoblastic MC3T3-E1 cells.

作者信息

Feres-Filho E J, Choi Y J, Han X, Takala T E, Trackman P C

机构信息

Department of Periodontology and Oral Biology, Boston University Goldman School of Graduate Dentistry, Massachusetts, USA.

出版信息

J Biol Chem. 1995 Dec 22;270(51):30797-803. doi: 10.1074/jbc.270.51.30797.

DOI:10.1074/jbc.270.51.30797
PMID:8530522
Abstract

The final enzymatic step required for collagen cross-linking is the extracellular oxidative deamination of peptidyl-lysine and -hydroxylysine residues by lysyl oxidase. A cross-linked collagenous extracellular matrix is required for bone formation. The goals of this study were to compare the transforming growth factor (TGF)-beta 1 regulation of lysyl oxidase enzyme activity and steady state mRNA levels to changes in COL1A1 mRNA levels in MC3T3-E1 osteoblastic cells. TGF-beta 1 increased steady state lysyl oxidase and COL1A1 mRNA levels in a dose- and time-dependent manner. The increase in lysyl oxidase mRNA levels was transient, peaking at 12 h and 8.8 times controls in cells treated with 400 pM TGF-beta 1. COL1A1 steady state mRNA levels increased maximally to 3.5-fold of controls. Development of increased lysyl oxidase enzyme activity was delayed and was of slightly lower magnitude than the increase in its mRNA levels. This suggested limiting post-translational processing of lysyl oxidase proenzyme. Pulse-labeling/immunoprecipitation studies demonstrated slow proenzyme secretion and proteolytic processing. Development and application of an independent assay for lysyl oxidase proenzyme proteolytic processing activity verified its proportionately lower stimulation by 400 pM TGF-beta 1. Thus, lysyl oxidase regulation by TGF-beta 1 in osteoblastic cell cultures occurs at both pre- and post-translational levels. This regulation is consistent with increased production of a collagenous extracellular matrix.

摘要

胶原蛋白交联所需的最后一个酶促步骤是赖氨酰氧化酶对肽基赖氨酸和羟赖氨酸残基进行细胞外氧化脱氨。骨形成需要交联的胶原细胞外基质。本研究的目的是比较转化生长因子(TGF)-β1对MC3T3-E1成骨细胞中赖氨酰氧化酶活性和稳态mRNA水平的调节与COL1A1 mRNA水平的变化。TGF-β1以剂量和时间依赖性方式增加稳态赖氨酰氧化酶和COL1A1 mRNA水平。赖氨酰氧化酶mRNA水平的增加是短暂的,在用400 pM TGF-β1处理的细胞中,在12小时达到峰值,是对照的8.8倍。COL1A1稳态mRNA水平最大增加到对照的3.5倍。赖氨酰氧化酶活性增加的发展延迟,且幅度略低于其mRNA水平的增加。这表明赖氨酰氧化酶原酶的翻译后加工受到限制。脉冲标记/免疫沉淀研究表明酶原分泌和蛋白水解加工缓慢。一种独立的赖氨酰氧化酶原酶蛋白水解加工活性测定方法的开发和应用证实了其受到400 pM TGF-β1的刺激程度较低。因此,TGF-β1在成骨细胞培养物中对赖氨酰氧化酶的调节发生在翻译前和翻译后水平。这种调节与胶原细胞外基质产量的增加一致。

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