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对患有致死性成骨不全症的双胞胎所培养的皮肤成纤维细胞中I型胶原蛋白的研究。

Studies on type I collagen in skin fibroblasts cultured from twins with lethal osteogenesis imperfecta.

作者信息

Galicka Anna, Wołczyński Sławomir, Gindzieński Andrzej

机构信息

Department of Medical Chemistry, Medical Academy of Białystok, 15-230 Białystok 8, Poland.

出版信息

Acta Biochim Pol. 2003;50(2):481-8.

Abstract

Studies on type I procollagen produced by skin fibroblasts cultured from twins with lethal type II of osteogenesis imperfecta (OI) showed that biosynthesis of collagen (measured by L-[5-(3)H]proline incorporation into proteins susceptible to the action of bacterial collagenase) was slightly increased as compared to the control healthy infant. SDS/PAGE showed that the fibroblasts synthesized and secreted only normal type I procollagen. Electrophoretic analysis of collagen chains and CNBr peptides showed the same pattern of electrophoretic migration as in the controls. The lack of posttranslational overmodification of the collagen molecule suggested a molecular defect near the amino terminus of the collagen helix. Digestion of OI type I collagen with trypsin at 30 degrees C for 5 min generated a shorter than normal alpha2 chain which melted at 36 degrees C. Direct sequencing of an asymmetric PCR product revealed a heterozygous single nucleotide change C-->G causing a substitution of histidine by aspartic acid in the alpha2 chain at position 92. Pericellular processing of type I procollagen by the twin's fibroblasts yielded a later appearance of the intermediate pC-alpha1(I) form as compared with control cells.

摘要

对来自患有致死性II型成骨不全症(OI)的双胞胎的皮肤成纤维细胞所产生的I型前胶原的研究表明,与对照健康婴儿相比,胶原蛋白的生物合成(通过L-[5-(3)H]脯氨酸掺入易受细菌胶原酶作用的蛋白质中来衡量)略有增加。SDS/PAGE显示成纤维细胞仅合成并分泌正常的I型前胶原。胶原链和CNBr肽的电泳分析显示出与对照相同的电泳迁移模式。胶原分子缺乏翻译后过度修饰表明在胶原螺旋的氨基末端附近存在分子缺陷。在30℃用胰蛋白酶消化OI I型胶原5分钟产生了一条比正常α2链短的链,该链在36℃变性。对不对称PCR产物的直接测序揭示了一个杂合单核苷酸变化C→G,导致α2链第92位的组氨酸被天冬氨酸取代。与对照细胞相比,双胞胎成纤维细胞对I型前胶原的细胞周加工产生中间pC-α1(I)形式的时间较晚。

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