Weber S, Engel J, Wiedemann H, Glanville R W, Timpl R
Eur J Biochem. 1984 Mar 1;139(2):401-10. doi: 10.1111/j.1432-1033.1984.tb08019.x.
The globular domain of collagen IV was solubilized by collagenase digestion from a mouse tumor, human placenta and bovine aorta and was purified by chromatographic methods. The materials show a unique, mainly non-collagenous amino acid composition and contain small amounts of glucosamine and galactosamine. The globular structures with Mr = 170 000 appear as a hexameric assembly originating from two collagen IV molecules. Subunits of this assembly are two different dimers Da and Db (Mr about 56 000) and monomers (Mr = 28 000). Their N-terminal amino acid sequences start with short triple-helical sequences, which overlap with the C-terminal triple helix of the alpha 1(IV) and alpha 2(IV) chain, demonstrating that the globule originates from the C terminus of collagen IV. Dimers arise from monomers by disulfide cross-linking (form Db) and/or formation of non-reducible cross-links (form Da). Reduction under non-denaturing conditions causes partial dissociation of the globule and of collagen IV dimers, indicating that reducible cross-links are formed between monomers of two different collagen IV molecules. Dissociation of the hexamer into the subunits can be achieved with 8 M urea, sodium dodecyl sulfate or in the pH range 2.5-4. The latter indicates that carboxyl groups are essential for association. Mixtures of the subunits (monomers and dimers) or purified dimers reassemble in neutral buffer into hexamers as shown by ultracentrifugation and electron microscopy. Reconstituted hexamers, however, dissociate in a much broader pH range than the native globules. Circular dichroic spectra indicate that the structure is more completely refolded from acid-treated than from urea-treated material. These data suggest that globules originating from monomers (as existing in single collagen IV molecules) are stabilized by the adjacent triple helix. Covalent cross-link formation stabilizes the globular structure and allows reconstitution in stoichiometric proportions.
通过胶原酶消化从小鼠肿瘤、人胎盘和牛主动脉中溶解出IV型胶原的球状结构域,并采用色谱方法进行纯化。这些物质呈现出独特的、主要是非胶原性的氨基酸组成,并且含有少量的氨基葡萄糖和半乳糖胺。分子量为170000的球状结构呈现为源自两个IV型胶原分子的六聚体组装形式。该组装体的亚基是两种不同的二聚体Da和Db(分子量约为56000)以及单体(分子量=28000)。它们的N端氨基酸序列起始于短的三螺旋序列,这些序列与α1(IV)和α2(IV)链的C端三螺旋重叠,表明该球状结构域源自IV型胶原的C端。二聚体通过二硫键交联(形成Db形式)和/或形成不可还原的交联(形成Da形式)由单体产生。在非变性条件下还原会导致球状结构域和IV型胶原二聚体部分解离,表明在两个不同IV型胶原分子的单体之间形成了可还原的交联。六聚体解离为亚基可以通过8M尿素、十二烷基硫酸钠或在pH值2.5 - 4范围内实现。后者表明羧基对于组装至关重要。亚基混合物(单体和二聚体)或纯化的二聚体在中性缓冲液中重新组装成六聚体,超速离心和电子显微镜观察证实了这一点。然而,重构的六聚体在比天然球状结构域更宽的pH范围内解离。圆二色光谱表明,与尿素处理的材料相比,酸处理的材料的结构能更完全地重新折叠。这些数据表明,源自单体(如单个IV型胶原分子中存在的)的球状结构域通过相邻的三螺旋得以稳定。共价交联的形成稳定了球状结构,并允许以化学计量比例进行重构。
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