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利用碳-13磁共振对软骨中蛋白聚糖的分子运动进行研究。

Investigation of molecular motion of proteoglycans in cartilage by 13C magnetic resonance.

作者信息

Torchia D A, Hasson M A, Hascall V C

出版信息

J Biol Chem. 1977 Jun 10;252(11):3617-25.

PMID:140875
Abstract

13C nmr spectral parameters were measured for intact bovine nasal cartilage tissue, the purified proteoglycan aggregate, and chondroitin 4-sulfate. A comparison of integrated intensities obtained for four different samples of fresh tissue with an ethylene glycol standard indicated that at least 80% of the total glycosaminoglycan carbons in the tissue contributed to the spectrum. This result was confirmed by intensity measurements obtained at 56 degrees on fresh tissue and at 37 degrees after extensive papain digestion of fresh tissue. Spin lattice relaxation times and nuclear Overhauser enhancements were analyzed in terms of the following models of molecular motion: (a) single correlation time; (b) log X2 distribution of correlation times; and (c) anisotropic motion. The analysis indicates that the segmental motions of glycosaminoglycan chains are characterized by a broad distribution of correlation times centered at about 50 ns. Slow motion contributions to glycosaminoglycan line widths were reduced by dipolar decoupling (gammaH2/2pi = 65 kHz). Collagen intensity was observed in dipolar decoupled spectra, but not in scalar decoupled spectra of intact tissue, showing that the type II collagen in cartilage undergoes anisotropic motion like the type I collagen in tendon. Only glycosaminoglycan resonances were observed in spectra of a solution of proteoglycan aggregate before and after chondroitinase digestion. After subsequent digestion with papain, protein resonances were observed. These results suggest that the protein portions of the proteoglycan aggregate structure, in contrast with the glycosaminoglycan chains, have restricted backbone mobility and consequently a defined backbone structure.

摘要

对完整的牛鼻软骨组织、纯化的蛋白聚糖聚集体和硫酸软骨素4进行了13C核磁共振光谱参数测量。用乙二醇标准品对四个不同新鲜组织样品获得的积分强度进行比较,结果表明组织中至少80%的总糖胺聚糖碳对光谱有贡献。在新鲜组织56℃时以及新鲜组织经木瓜蛋白酶广泛消化后37℃时获得的强度测量结果证实了这一结果。根据以下分子运动模型分析了自旋晶格弛豫时间和核Overhauser增强:(a)单相关时间;(b)相关时间的对数X2分布;(c)各向异性运动。分析表明,糖胺聚糖链的节段运动具有以约50纳秒为中心的宽相关时间分布特征。通过偶极去耦(γH2/2π = 65千赫)减少了对糖胺聚糖线宽的慢运动贡献。在偶极去耦光谱中观察到了胶原蛋白强度,但在完整组织的标量去耦光谱中未观察到,这表明软骨中的II型胶原蛋白与肌腱中的I型胶原蛋白一样经历各向异性运动。在软骨素酶消化前后的蛋白聚糖聚集体溶液光谱中仅观察到糖胺聚糖共振。在用木瓜蛋白酶随后消化后,观察到了蛋白质共振。这些结果表明,与糖胺聚糖链相比,蛋白聚糖聚集体结构的蛋白质部分具有受限的主链流动性,因此具有明确的主链结构。

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Investigation of molecular motion of proteoglycans in cartilage by 13C magnetic resonance.利用碳-13磁共振对软骨中蛋白聚糖的分子运动进行研究。
J Biol Chem. 1977 Jun 10;252(11):3617-25.
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