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前胶原的二硫键结合性质以及延伸肽段在分子组装中的作用。

The disulphide-bonded nature of procollagen and the role of the extension peptides in the assembly of the molecule.

作者信息

Harwood R, Merry A H, Woolley D E, Grant M E, Jackson D S

出版信息

Biochem J. 1977 Feb 1;161(2):405-18. doi: 10.1042/bj1610405.

DOI:10.1042/bj1610405
PMID:192195
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1164518/
Abstract
  1. The molecular weights of chick tendon and cartilage procollagens, and their constituent polypeptides, were determined by gel filtration and gel electrophoresis. The values obtained are in good agreement and indicate that the mol.wts. of the secreted procollagens (types I and II) and their individual pro-alpha-chains are of the order of 405 000-445 000 and 137 000-145 000 respectively.2. Digestion of tendon procollagen with human rheumatoid synovial collagenase gave products consistent with the presence of large non-helical peptide extensions at both N-and C-termini. Electrophoretic analysis gave apparent mol.wts. of 17 500 and 36 000 for the respective N- and C-terminal extensions of pro-alpha1(I)-and pro-alpha2-chains, and inter-chain disulphide bonds were restricted to the C-terminal location. 3. During the biosynthesis of procollagen by tendon and cartilage cells a close correlation was observed between the extent of inter-chain disulphide bonding and the proportion of procollagen polypeptides having a triple-helical conformation. These processes appeared to commence in the rough endoplasmic reticulum and be completed in the smooth endoplasmic reticulum, but the rate at which they occur in cartilage cells is markedly slower than that found in tendon cells. 4. When the intracellular [14C]procollagen polypeptides present in the rough-endoplasmic-reticulum fractions of tendon and cartilage cells were analysed under non-reducing conditions on agarose/polyacrylamide composite gels, no significant pools of dimeric intermediates were detected. 5. In both cell types, inter-chain disulphide-bond formation occurred even when hydroxylation, and hence triple-helix formation, was inhibited. The presence of pro-alpha1- and pro-alpha2-components in a ratio of 2:1 in the disulphide-linked unhydroxylated procollagen isolated from tendon cells demonstrated that correct chain association occurs in the absence of hydroxylation. This observation is consistent with a model for the assembly of pro-gamma112-chains in which the recognition and selection of pro-alpha1-and pro-alpha2-chains in a 2:1 ratio are directed by the non-helical C-terminal extension peptides of tendon procollagen.
摘要
  1. 通过凝胶过滤和凝胶电泳测定了鸡肌腱和软骨前胶原及其组成多肽的分子量。所得数值吻合良好,表明分泌型前胶原(I型和II型)及其各自的前α链的分子量分别约为405000 - 445000和137000 - 145000。

  2. 用人类风湿性滑膜胶原酶消化肌腱前胶原得到的产物与在N端和C端均存在大的非螺旋肽延伸的情况相符。电泳分析得出前α1(I)链和前α2链各自N端和C端延伸的表观分子量分别为17500和36000,链间二硫键局限于C端位置。

  3. 在肌腱和软骨细胞合成前胶原的过程中,观察到链间二硫键结合程度与具有三螺旋构象的前胶原多肽比例之间存在密切相关性。这些过程似乎始于粗面内质网并在滑面内质网中完成,但它们在软骨细胞中的发生速率明显慢于在肌腱细胞中的速率。

  4. 当在非还原条件下在琼脂糖/聚丙烯酰胺复合凝胶上分析存在于肌腱和软骨细胞粗面内质网部分中的细胞内[14C]前胶原多肽时,未检测到明显的二聚体中间体库。

  5. 在两种细胞类型中,即使羟基化以及因此的三螺旋形成受到抑制,链间二硫键仍会形成。从肌腱细胞分离的二硫键连接的未羟基化前胶原中前α1和前α2组分以2:1的比例存在,这表明在没有羟基化的情况下也会发生正确的链缔合。这一观察结果与前γ112链组装模型一致,在该模型中,前α1链和前α2链以2:1比例的识别和选择由肌腱前胶原的非螺旋C端延伸肽指导。

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1
The disulphide-bonded nature of procollagen and the role of the extension peptides in the assembly of the molecule.前胶原的二硫键结合性质以及延伸肽段在分子组装中的作用。
Biochem J. 1977 Feb 1;161(2):405-18. doi: 10.1042/bj1610405.
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The synthesis and secretion of cartilage procollagen.软骨前胶原的合成与分泌。
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Biochem J. 1976 Apr 15;156(1):81-90. doi: 10.1042/bj1560081.
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Further evidence for a transport form of collagen. Its extrusion and extracellular conversion to tropocollagen in embryonic tendon.胶原蛋白转运形式的进一步证据。其在胚胎肌腱中的挤出及细胞外转化为原胶原蛋白。
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Collagen biosynthesis: synthesis and secretion of a high molecular weight collagen precursor (procollagen).胶原蛋白生物合成:高分子量胶原蛋白前体(前胶原)的合成与分泌。
Proc Natl Acad Sci U S A. 1971 Nov;68(11):2638-42. doi: 10.1073/pnas.68.11.2638.
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Molecular weight determination of protein-dodecyl sulfate complexes by gel electrophoresis in a discontinuous buffer system.在不连续缓冲系统中通过凝胶电泳测定蛋白质 - 十二烷基硫酸盐复合物的分子量
J Biol Chem. 1971 Oct 25;246(20):6328-34.
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