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Surface Ultrastructure of Collagen Fibrils and Their Association With Proteoglycans in Human Cornea and Sclera by Atomic Force Microscopy and Energy-filtering Transmission Electron Microscopy

 

作者: Atsuko Miyagawa,   Miya Kobayashi,   Yoshikazu Fujita,   Ossama Hamdy,   Koji Hirano,   Makoto Nakamura,   Yozo Miyake,  

 

期刊: Cornea  (OVID Available online 2001)
卷期: Volume 20, issue 6  

页码: 651-656

 

ISSN:0277-3740

 

年代: 2001

 

出版商: OVID

 

关键词: Collagen fibrils;Proteoglycans;Keratan sulfate;Human cornea;Sclera

 

数据来源: OVID

 

摘要:

Purpose.We aimed to investigate the possible association of proteoglycans with D-periodic collagen fibrils in the human cornea and sclera, using energy-filtering transmission electron microscopy (EF-TEM) and atomic force microscopy (AFM).Methods.Human cornea and sclera were digested with keratanase to eliminate keratan sulfate proteoglycans (KSPGs). For EF-TEM observation, surface proteoglycans were detected by cupromeronic blue (CB) staining. For AFM observation, cornea and sclera were treated with sodium hydroxide before and after keratanase digestion, and the surface topology of collagen fibrils was analyzed.Results.With CB staining, numerous CB-positive short filaments of surface proteoglycans (proteoglycan filaments) were observed in the interfibrillar spaces of cornea and sclera associated with collagen fibrils. AFM imaging showed that the depth and periodicity of D-periodic collagen fibrils in keratanase-treated corneal collagens were deeper and more regular than in untreated ones. Moreover, the depth and periodicity of keratanase-untreated corneal collagens were shallow and irregular in comparison with keratanase-untreated scleral collagens. On the other hand, there was no difference in depth or regularity between keratanase-treated and -untreated scleral collagen fibrils. Using AFM imaging, additional thin grooves sub-bands were detected on the surface of keratanase-treated corneal collagen fibrils. The grooves were not detected in keratanase-untreated collagen fibrils nor in scleral collagen fibrils with or without keratanase digestion. Comparing densitometry waves, the grooves of D-periodic corneal collagen sub-bands corresponded to a and c bands.Conclusion.Using AFM and EF-TEM to study corneal and scleral collagen fibrils and their association with proteoglycans, we conclude that KSPG is found in ample amounts in the human cornea in comparison with sclera. Moreover, we topologically detected KSPG attached to a and c bands of collagen fibrils.

 

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