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兔晶状体囊蛋白聚糖分布和大小不均一。

Uneven distribution and size of rabbit lens capsule proteoglycans.

作者信息

Landemore G, Stefani P, Quillec M, Lecoq-Guilbert P, Billotte C, Izard J

机构信息

Laboratoire d'Histologie et Biologie Cellulaire, UFR de Médecine, Université de Caen-Basse Normandie, Caen, France.

出版信息

Histochem J. 1999 Mar;31(3):161-7. doi: 10.1023/a:1003598919867.

Abstract

To document the ultrastructural distribution of lens capsule proteoglycans, rabbit lens capsules were fixed and stained overnight in 50 mM sodium acetate, pH 5.6, containing 2.5% glutaraldehyde, 0.2% Cuprolinic Blue and 0.2 M MgCl2. They were rinsed, stained with 1% aqueous sodium tungstate, embedded in Epon, sectioned (60 nm), and examined with an electron microscope at 60 kV. Proteoglycan-Cuprolinic Blue complexes mainly appeared as networks of small electron-dense filaments throughout the posterior and anterior capsules. The posterior capsule was a single layer with a network of small proteoglycan filaments gradually decreasing in size from the humoral side (90 x 10 nm) to the lenticular side (30 x 8 nm). The humoral side of the anterior capsule had a thin lamina (400 nm) containing large (180 x 40 nm), very electron-dense proteoglycan-Cuprolinic Blue complexes plus small proteoglycans. Below this lamina, the complexes were only seen as filaments slightly smaller than those in the corresponding area of the posterior capsule. Cuprolinic Blue binding of the anterior and posterior lens capsules revealed differences in the size and distribution of their sulphated proteoglycans which do not correspond to the patterns of their immunoreactivity with anti-heparan sulphate proteoglycan. The humoral lamina in the anterior capsules, with large proteoglycan structures, might be a distinct structural and functional compartment.

摘要

为记录晶状体囊蛋白聚糖的超微结构分布,将兔晶状体囊固定于含2.5%戊二醛、0.2%铜试剂蓝和0.2 M氯化镁的50 mM醋酸钠(pH 5.6)中过夜染色。冲洗后,用1%钨酸钠水溶液染色,包埋于环氧树脂中,切片(60 nm),并在60 kV下用电子显微镜检查。蛋白聚糖 - 铜试剂蓝复合物主要呈现为贯穿后囊和前囊的小电子致密细丝网络。后囊为单层,小蛋白聚糖细丝网络从体液侧(90×10 nm)到晶状体侧(30×8 nm)尺寸逐渐减小。前囊的体液侧有一层薄的板层(400 nm),含有大的(180×40 nm)、电子密度非常高的蛋白聚糖 - 铜试剂蓝复合物以及小蛋白聚糖。在该板层下方,复合物仅呈现为比后囊相应区域稍小的细丝。前囊和后囊的铜试剂蓝结合显示出其硫酸化蛋白聚糖在大小和分布上的差异,这与它们与抗硫酸乙酰肝素蛋白聚糖的免疫反应模式不对应。前囊中具有大蛋白聚糖结构的体液板层可能是一个独特的结构和功能区室。

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