Filla Mark S, Liu Xuyang, Nguyen Thai D, Polansky Jon R, Brandt Curtis R, Kaufman Paul L, Peters Donna M
Department of Ophthalmology and Visual Sciences, University of Wisconsin, Madison, Wisconsin 53706, USA.
Invest Ophthalmol Vis Sci. 2002 Jan;43(1):151-61.
To determine whether trabecular meshwork-inducible glucocorticoid response/myocilin (TIGR/MYOC) protein associates with the extracellular matrix (ECM) of human trabecular meshwork (HTM) cells.
The extracellular localization of TIGR/MYOC was examined by immunofluorescence microscopy in HTM cultures treated with and without dexamethasone and ascorbate and in a transformed HTM cell line, TM-1, transiently transfected with TIGR/MYOC cDNA. Antibodies to TIGR/MYOC, fibronectin, laminin, type IV collagen, or thrombospondin were used to determine the extracellular localization of TIGR/MYOC. Solid phase binding assays using 125I-recombinant TIGR/MYOC and types I and IV collagens, fibronectin, and laminin were done to examine the association of TIGR/MYOC with these proteins and to identify a specific TIGR/MYOC binding site within fibronectin. The domains of fibronectin tested were the fibrin/collagen binding domain, the RGD domain, and the Heparin II (Hep II) domain.
TIGR/MYOC colocalized with fibronectin, laminin, and type IV collagen, but not thrombospondin in both dexamethasone and dexamethasone/ascorbate-treated HTM cultures and in TM-1 cultures transfected with TIGR/MYOC cDNA. In solid phase binding assays, 125I-TIGR/MYOC bound fibronectin but not laminin or type IV collagen. Binding to fibronectin could be competed with excess TIGR/MYOC or fibronectin. Specific binding was found for the Hep II domain of fibronectin.
TIGR/MYOC can associate with components of the ECM via interactions with the Hep II domain of fibronectin. The interactions with the Hep II domain of fibronectin could alter cell-matrix interactions in the TM and provides an interesting lead to explore the role(s) of TIGR/MYOC in both steroid-induced and primary open angle glaucoma.
确定小梁网诱导性糖皮质激素反应蛋白/肌纤凝蛋白(TIGR/MYOC)是否与人小梁网(HTM)细胞的细胞外基质(ECM)相关联。
通过免疫荧光显微镜检查TIGR/MYOC在接受和未接受地塞米松及抗坏血酸处理的HTM培养物中的细胞外定位,以及在瞬时转染TIGR/MYOC cDNA的转化HTM细胞系TM-1中的细胞外定位。使用针对TIGR/MYOC、纤连蛋白、层粘连蛋白、IV型胶原或血小板反应蛋白的抗体来确定TIGR/MYOC的细胞外定位。使用125I重组TIGR/MYOC与I型和IV型胶原、纤连蛋白及层粘连蛋白进行固相结合试验,以检测TIGR/MYOC与这些蛋白质的关联,并确定纤连蛋白内的特定TIGR/MYOC结合位点。所检测的纤连蛋白结构域为纤维蛋白/胶原结合结构域、RGD结构域和肝素II(Hep II)结构域。
在接受地塞米松及地塞米松/抗坏血酸处理的HTM培养物以及转染TIGR/MYOC cDNA的TM-1培养物中,TIGR/MYOC与纤连蛋白、层粘连蛋白和IV型胶原共定位,但不与血小板反应蛋白共定位。在固相结合试验中,125I-TIGR/MYOC结合纤连蛋白,但不结合层粘连蛋白或IV型胶原。与纤连蛋白的结合可被过量的TIGR/MYOC或纤连蛋白竞争。发现TIGR/MYOC与纤连蛋白的Hep II结构域存在特异性结合。
TIGR/MYOC可通过与纤连蛋白的Hep II结构域相互作用而与ECM成分相关联。与纤连蛋白的Hep II结构域的相互作用可能改变小梁网中的细胞-基质相互作用,并为探索TIGR/MYOC在类固醇诱导性和原发性开角型青光眼中的作用提供了有趣的线索。
Zotero 插件