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Polymeric C-terminal cross-linked material from type-I collagen. A modified method for purification, anomalous behaviour on gel filtration, molecular weight estimation, carbohydrate content and lipid content

机译:来自I型胶原的聚合C末端交联材料。一种改进的纯化方法,凝胶过滤的异常行为,分子量估算,碳水化合物含量和脂质含量

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pPolymeric cross-linked C-terminal peptide material (poly-alpha 1CB6) from mature bovine tendon type-I collagen was prepared and purified by a modification of the method previously described [Light & Bailey (1980) Biochem. J. 185, 373-381]. Poly-alpha 1CB6 was shown to exhibit concentration-dependent aggregation effects on gel filtration due to interaction with a filtration medium. The material had an amino acid content that was very similar to a mixture of alpha 1CB6 and alpha 1CB5. The material was shown to be polydisperse with a mol.wt. range of 50 000-350 000, but chromatographic fractions were relatively homogeneous over this molecular weight range with respect to amino-acid composition. The heterogeneity of the material was not due to incomplete CNBr peptide cleavage, as poly-alpha 1CB6 did not contain detectable quantities of methionine. The material showed no discrete bands on sodium dodecyl sulphate/polyacrylamide-gel electrophoresis but gave a constant blue stain throughout the molecular weight range described above. Lipid analysis showed that the partially purified material contained elevated levels of stearate when compared to the crude CNBr-digested starting material. This may indicate the specific association of a stearic-acid-rich lipid with the peptide material. On carbohydrate analysis poly-alpha 1CB6 was shown to contain only galactose and glucose at levels of 0.72 and 0.28% respectively. The carbohydrate and amino acid analyses indicated that (alpha 1CB6)2-(alpha 1CB5)1 may be the basic cross-linked structural unit of poly-alpha 1CB6)2-(alpha 1CB5)1 units, although the carbohydrate analysis indicated that the higher molecular weight oligomers may be enriched in alpha 1CB6./p
机译:制备来自成熟的I型牛腱胶原的聚合物交联的C-末端肽材料(聚-α1CB6),并通过前述方法的改进[Light& Co.Chem.Soc。,2006,6,5,5]。 Bailey(1980)Biochem。 J. 185,373-381]。由于与过滤介质的相互作用,聚α1CB6对凝胶过滤表现出浓度依赖性的聚集效应。该物质的氨基酸含量与α1CB6和α1CB5的混合物非常相似。该材料显示为具有分子量的多分散体。分子量范围为50000-350000,但是在该分子量范围内,相对于氨基酸组成,色谱分离部分是相对均匀的。该材料的异质性不是由于CNBr肽裂解不完全所致,因为聚α1CB6不包含可检测量的蛋氨酸。该材料在十二烷基硫酸钠/聚丙烯酰胺-凝胶电泳上没有显示离散的带,但在上述分子量范围内均显示出恒定的蓝色斑点。脂质分析表明,与粗制CNBr消化的起始原料相比,部分纯化的物质含有较高含量的硬脂酸盐。这可能表明富含硬脂酸的脂质与肽材料的特定结合。在碳水化合物分析中,聚α1CB6仅含半乳糖和葡萄糖,含量分别为0.72和0.28%。碳水化合物和氨基酸分析表明,(α1CB6)2-(α1CB5)1可能是聚-α1CB6)2-(α1CB5)1单元的基本交联结构单元,尽管碳水化合物分析表明,较高分子量的低聚物可能富含α1CB6。

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