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糖皮质激素对胶原蛋白代谢的调节。地塞米松对鸡胚成纤维细胞和软骨细胞中胶原蛋白生物合成的受体介导作用。

Modulation of collagen metabolism by glucocorticoids. Receptor-mediated effects of dexamethasone on collagen biosynthesis in chick embryo fibroblasts and chondrocytes.

作者信息

Oikarinen A I, Vuorio E I, Zaragoza E J, Palotie A, Chu M L, Uitto J

机构信息

Department of Dermatology, University of Oulu, Finland.

出版信息

Biochem Pharmacol. 1988 Apr 15;37(8):1451-62. doi: 10.1016/0006-2952(88)90006-8.

Abstract

The steroid modulation of collagen metabolism was studied by injecting chick embryos with dexamethasone in vivo, and collagen synthesis was subsequently assayed by pulse-labeling the tissue with [14C]proline in vitro. The synthesis of [14C]hydroxyproline in tendons and sterna from chick embryos treated with dexamethasone was markedly reduced as compared with untreated controls. The inhibition of [3H]hydroxyproline synthesis was accompanied by a similar reduction in type I and II procollagen mRNA levels, as detected by Northern blot and dot blot hybridizations with chick pro alpha 1(I), pro alpha 2(I) and pro alpha 1(II) sequence specific cDNAs. The reduction in type II procollagen mRNA level was shown to be dose dependent. Control experiments indicated that the post-translational hydroxylation of prolyl residues was only slightly decreased in dexamethasone treated animals, and that the specific activity of the intracellular free proline pool and the intracellular degradation of collagen were unchanged. To address the mechanisms of the inhibition of collagen biosynthesis, specific binding of dexamethasone to glucocorticoid receptors in chick embryo tendon and cartilage cells was studied in a whole cell assay using [3H]dexamethasone as the ligand. Matrix-free tendon and cartilage cells had approximately 19,000 and 15,000 receptor sites per cell, respectively, and the binding affinities (Kd) for dexamethasone in tendon and cartilage cells were 2.9 x 10(-9) and 2.3 x 10(-9) M. Comparable values were obtained using a cytosol binding assay. The nuclear binding of dexamethasone in tendon and cartilage cells were similar. The results suggest that the dexamethasone-induced inhibition of collagen production is primarily due to decreased levels of functional procollagen mRNA, possibly resulting from receptor-mediated inhibition of the gene expression on the transcriptional level.

摘要

通过在体内给鸡胚注射地塞米松来研究类固醇对胶原蛋白代谢的调节作用,随后通过在体外用[14C]脯氨酸对组织进行脉冲标记来测定胶原蛋白的合成。与未处理的对照组相比,用地塞米松处理的鸡胚的肌腱和胸骨中[14C]羟脯氨酸的合成明显减少。通过用鸡原α1(I)、原α2(I)和原α1(II)序列特异性cDNA进行Northern印迹和斑点印迹杂交检测,[3H]羟脯氨酸合成的抑制伴随着I型和II型前胶原mRNA水平的类似降低。II型前胶原mRNA水平的降低显示为剂量依赖性。对照实验表明,在地塞米松处理的动物中,脯氨酰残基的翻译后羟基化仅略有降低,并且细胞内游离脯氨酸池的比活性和胶原蛋白的细胞内降解未发生变化。为了探讨胶原蛋白生物合成抑制的机制,使用[3H]地塞米松作为配体,在全细胞测定中研究了地塞米松与鸡胚肌腱和软骨细胞中糖皮质激素受体特异性结合。无基质的肌腱和软骨细胞每细胞分别约有19,000和15,000个受体位点,并且地塞米松在肌腱和软骨细胞中的结合亲和力(Kd)分别为2.9×10(-9)和2.3×10(-9)M。使用细胞质结合测定获得了可比的值。地塞米松在肌腱和软骨细胞中的核结合相似。结果表明,地塞米松诱导的胶原蛋白产生抑制主要是由于功能性前胶原mRNA水平降低,这可能是由于受体介导的转录水平基因表达抑制所致。

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