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Additive effects of extracellular matrix proteins and platelet derived mitogens on human retinal pigment epithelial cell proliferation and contraction

 

作者: SmithL.,   RichardsonP.,   ParsonsM. A.,   RennieI. G.,   BensonM.,   MacneilS.,  

 

期刊: Current Eye Research  (Taylor Available online 1996)
卷期: Volume 15, issue 7  

页码: 739-748

 

ISSN:0271-3683

 

年代: 1996

 

DOI:10.3109/02713689609003457

 

出版商: Taylor&Francis

 

关键词: retinal pigment epithelial (RPE cells);extracellular matrix (ECM);growth factors;proliferation;contraction;human;cell culture

 

数据来源: Taylor

 

摘要:

Purpose.In proliferative vitreoretinopathy (PVR) retinal pigment epithelial (RPE) cells are thought to synthesise and interact with extracellular matrix (ECM) proteins to form fibrocellular membranes attached to the retina, which the cells then progressively contract detaching the retina. Haemorrhage into the eye is an exacerbating factor in the pathology. To investigate some of the possible interactions between ECM proteins, platelet mitogens and RPE cells in this study, we examined the combined effect of platelet derived mitogens and ECM proteins on RPE cell proliferation and contraction.Methods.Cells were cultured on a range of individual ECM proteins as well as on the ECM deposited by normal vitreous fluid and exposed to platelet mitogens. Effects on cell proliferation and cell detachment from these substrates and tissue culture plastic were examined.Results.We report additive/synergistic effects of platelet mitogens (PDGF and TGFb) as well as bFGF, with ECM proteins (laminin, fibronectin, collagen 1 and vitreous-deposited ECM) on RPE proliferation. Further we report stimulation of RPE cell contraction on vitreous proteins when exposed to serum prepared from platelet-rich plasma. In this context it was noticeable that it was cells grown on vitreous matrix plus pigment rather than cells grown on clear vitreous that exhibited this behaviour.Conclusions.This study supports a combined action of platelet mitogens and matrix proteins in inducing RPE cell proliferation and contractility and provides a simplein vitromodel of some of the late stages of PVR.

 

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