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通过mRNA的可变剪接,II型(软骨)前胶原氨基末端前肽中富含半胱氨酸结构域的差异表达。

Differential expression of a cysteine-rich domain in the amino-terminal propeptide of type II (cartilage) procollagen by alternative splicing of mRNA.

作者信息

Ryan M C, Sandell L J

机构信息

Department of Biochemistry, Rush-Presbyterian-St. Luke's Medical Center, Chicago, Illinois 60612.

出版信息

J Biol Chem. 1990 Jun 25;265(18):10334-9.

PMID:2355003
Abstract

Type II collagen, like other fibrillar collagens, is synthesized as a procollagen containing amino (NH2)-and carboxyl (COOH)-terminal extension peptides. Based on cDNA cloning of human (Baldwin, C. T., Reginato, A. M., Smith, C., Jimenez, S. A., and Prockop, D. J. (1989) Biochem. J. 262, 521-528) and rat (Kohno, K., Martin, G. R., and Yamada, Y. (1984) J. Biol. Chem. 259, 13668-13673) type II procollagen, it was concluded that much of the NH2-terminal propeptide seen in pro-alpha 1(I) was missing. Analysis of human genomic clones for type II collagen revealed an additional exon encoding a 69-amino acid cysteine-rich domain in the NH2-terminal propeptide. This exon (exon 2) is expressed in the mRNA population of chondrocytes isolated from human fetal skeleton and notochord, juvenile costal cartilage, and bovine articular cartilage. Oligonucleotide probes spanning specific exon boundaries were used to detect two populations of procollagen mRNA by Northern blot analysis. Amplification of cDNA templates using polymerase chain reaction provided direct evidence for two distinct pro-alpha 1(II) collagen mRNAs. DNA sequence analysis showed that the two mRNAs resulted from the alternative splicing of exon 2. The protein domain encoded by exon 2 is conserved between the fibrillar collagens and two other extracellular matrix proteins, thrombospondin and von Willebrand factor. In fibrillar collagens, this protein domain may play a regulatory role in fibrillogenesis and feedback inhibition of collagen biosynthesis. Consequently, the differential expression of this protein domain could alter the biosynthesis or fibril formation of type II collagen. In addition, the expression of exon 2 may be a marker for a distinct population of chondrocytes.

摘要

与其他纤维状胶原蛋白一样,II型胶原蛋白最初合成时是一种包含氨基(NH2)和羧基(COOH)末端延伸肽的前胶原蛋白。基于人(鲍德温,C.T.,雷吉纳托,A.M.,史密斯,C.,希门尼斯,S.A.,和普罗科普,D.J.(1989年)《生物化学杂志》262卷,521 - 528页)和大鼠(小川,K.,马丁,G.R.,和山田,Y.(1984年)《生物化学杂志》259卷,13668 - 13673页)II型前胶原蛋白的cDNA克隆,得出的结论是前α1(I)中所见的大部分NH2末端前肽缺失。对人II型胶原蛋白基因组克隆的分析揭示了一个额外的外显子,其编码NH2末端前肽中一个富含69个氨基酸的半胱氨酸结构域。这个外显子(外显子2)在从人胎儿骨骼和脊索、青少年肋软骨以及牛关节软骨分离的软骨细胞的mRNA群体中表达。通过Northern印迹分析,使用跨越特定外显子边界的寡核苷酸探针来检测前胶原蛋白mRNA的两个群体。利用聚合酶链反应对cDNA模板进行扩增,为两种不同的前α1(II)胶原蛋白mRNA提供了直接证据。DNA序列分析表明,这两种mRNA是由外显子2的可变剪接产生的。外显子2编码的蛋白质结构域在纤维状胶原蛋白与另外两种细胞外基质蛋白——血小板反应蛋白和血管性血友病因子之间是保守的。在纤维状胶原蛋白中,这个蛋白质结构域可能在纤维形成以及胶原蛋白生物合成的反馈抑制中发挥调节作用。因此,这个蛋白质结构域的差异表达可能会改变II型胶原蛋白的生物合成或纤维形成。此外,外显子2的表达可能是一种独特软骨细胞群体的标志物。

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