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来自牛巩膜的硫酸皮肤素蛋白聚糖的自我缔合。

Self-association of dermatan sulphate proteoglycans from bovine sclera.

作者信息

Cöster L, Fransson L A, Sheehan J, Nieduszynski I A, Phelps C F

出版信息

Biochem J. 1981 Aug 1;197(2):483-90. doi: 10.1042/bj1970483.

Abstract
  1. Two proteodermatan sulphate fractions (I and II) from bovine sclera were studied by gel chromatography, light-scattering and ultracentrifugation under various conditions. 2. Gel chromatography of proteoglycans in the absence or presence of hyaluronate was performed under associative conditions. No effect on the elution profile was noted. 3. Ultracentrifugation experiments (sedimentation-velocity and sedimentation-equilibrium) with proteoglycan I and II in 6 M-guanidine hydrochloride gave molecular weights (Mw) of 160000-220000 and 70000-100000 respectively. As the protein contents were 45% and 60% respectively, it may be calculated that proteoglycan I contained four to five side chains, whereas proteoglycan II contained one or two. Sedimentation-equilibrium runs performed in 0.15 M-NaCl gave an apparent molecular weight (Mw) of 500000-800000 for proteoglycan I and 90000-110000 for proteoglycan II. 4. In light-scattering experiments both proteoglycans I and II yielded high particle weights in 0.15 M-NaCl (3.1 X 10(6) and 3.4 X 10(6) daltons respectively). In the presence of 6 M-guanidine hydrochloride the molecular weights decreased to 410000 and 130000 respectively. The particle weights in 0.15 M-NaCl were not altered by the addition of hyaluronate or hyaluronate oligosaccharides. 5. The dermatan sulphate side chains of scleral proteoglycans (L-iduronate/D-glucuronate ratio 7:13) gave a particle weight of 100000 daltons in 0.15 M-NaCl. In 1.00 M-KCl/0.02M-EDTA the molecular weight was 24000. Addition of free scleral dermatan sulphate chains to a solution of proteoglycan II promoted further multimerization of the macromolecule.
摘要
  1. 采用凝胶色谱法、光散射法和超速离心法,在不同条件下对牛巩膜中的两种硫酸皮肤素蛋白聚糖组分(I和II)进行了研究。2. 在缔合条件下,对有无透明质酸存在时的蛋白聚糖进行了凝胶色谱分析。未观察到对洗脱曲线有影响。3. 在6M盐酸胍中对蛋白聚糖I和II进行超速离心实验(沉降速度和沉降平衡),得到的分子量(Mw)分别为160000 - 220000和70000 - 100000。由于蛋白质含量分别为45%和60%,可以计算出蛋白聚糖I含有四到五个侧链,而蛋白聚糖II含有一或两个侧链。在0.15M氯化钠中进行的沉降平衡实验得出,蛋白聚糖I的表观分子量(Mw)为500000 - 800000,蛋白聚糖II为90000 - 110000。4. 在光散射实验中,蛋白聚糖I和II在0.15M氯化钠中都产生了较高的颗粒重量(分别为3.1×10⁶和3.4×10⁶道尔顿)。在6M盐酸胍存在下,分子量分别降至410000和130000。在0.15M氯化钠中加入透明质酸或透明质酸寡糖后,颗粒重量未发生改变。5. 巩膜蛋白聚糖的硫酸皮肤素侧链(艾杜糖醛酸/葡萄糖醛酸比例为7:13)在0.15M氯化钠中的颗粒重量为100000道尔顿。在1.00M氯化钾/0.02M乙二胺四乙酸中,分子量为24000。向蛋白聚糖II溶液中添加游离的巩膜硫酸皮肤素链会促进大分子的进一步多聚化。

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