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牛关节软骨培养物中蛋白聚糖的周转

Turnover of proteoglycans in cultures of bovine articular cartilage.

作者信息

Campbell M A, Handley C J, Hascall V C, Campbell R A, Lowther D A

出版信息

Arch Biochem Biophys. 1984 Oct;234(1):275-89. doi: 10.1016/0003-9861(84)90350-3.

Abstract

Proteoglycans in cultures of adult bovine articular cartilage labeled with [35S]sulfate after 5 days in culture and maintained in medium containing 20% fetal calf X serum had longer half-lives (average 11 days) compared with those of the same tissue maintained in medium alone (average 6 days). The half-lives of proteoglycans in cultures of calf cartilage labeled after 5 days in culture and maintained in medium with serum were considerably longer (average 21 days) compared to adult cartilage. If 0.5 mM cycloheximide was added to the medium of cultures of adult cartilage, or the tissue was maintained at 4 degrees C after labeling, the half-lives of the proteoglycans were greater, 24 and greater than 300 days, respectively. Analyses of the radiolabeled proteoglycans remaining in the matrix of the tissue immediately after labeling the tissue and at various times in culture revealed two main populations of proteoglycans; a large species eluting with Kav of 0.21-0.24 on Sepharose CL-2B, of high bouyant density and able to form aggregates with hyaluronate, and a small species eluting with a Kav of 0.63-0.70 on Sepharose CL-2B, of low buoyant density, containing only chondroitin sulfate chains, and unable to form aggregates with hyaluronate. The larger proteoglycan had shorter half-lives than the smaller proteoglycan; in cartilage maintained with serum, the half-lives were 9.8 and 14.5 days, respectively. Labeling cartilage with both [3H]leucine and [35S]sulfate showed the small proteoglycan to be a separate synthetic product. The size distribution of 35S-labeled proteoglycans lost into the medium was shown to be polydisperse on Sepharose CL-2B, the majority eluting with a Kav of 0.27 to 0.35, of high buoyant density, and unable to aggregate with hyaluronate. The size distribution of glycosaminoglycans from 35S-labeled proteoglycans appearing in the medium did not differ from that associated with labeled proteoglycans remaining in the matrix.

摘要

成年牛关节软骨培养物中的蛋白聚糖,在培养5天后用[35S]硫酸盐标记,并维持在含有20%胎牛血清的培养基中,与仅维持在培养基中的相同组织相比,其半衰期更长(平均11天)(平均6天)。与成年软骨相比,培养5天后标记并维持在含血清培养基中的小牛软骨培养物中蛋白聚糖的半衰期长得多(平均21天)。如果向成年软骨培养物的培养基中加入0.5 mM环己酰亚胺,或者在标记后将组织维持在4℃,蛋白聚糖的半衰期会更长,分别为24天和超过300天。在标记组织后立即以及在培养的不同时间对组织基质中残留的放射性标记蛋白聚糖进行分析,发现了两种主要的蛋白聚糖群体;一种大分子量的在Sepharose CL - 2B上以Kav 0.21 - 0.24洗脱,具有高浮力密度且能够与透明质酸形成聚集体,另一种小分子量的在Sepharose CL - 2B上以Kav 0.63 - 0.70洗脱,具有低浮力密度,仅含有硫酸软骨素链,且不能与透明质酸形成聚集体。较大的蛋白聚糖比较小的蛋白聚糖半衰期短;在含血清的软骨中,半衰期分别为9.8天和14.5天。用[3H]亮氨酸和[35S]硫酸盐同时标记软骨表明,小蛋白聚糖是一种单独的合成产物。在Sepharose CL - 2B上,释放到培养基中的35S标记蛋白聚糖的大小分布显示为多分散,大多数以Kav为0.27至0.35洗脱,具有高浮力密度,且不能与透明质酸聚集。培养基中出现的35S标记蛋白聚糖的糖胺聚糖的大小分布与基质中残留的标记蛋白聚糖的糖胺聚糖的大小分布没有差异。

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