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Matrix metalloproteinase-1 localization in the normal human uveoscleral outflow pathway.

机译:基质金属蛋白酶-1定位在正常人的葡萄膜巩膜流出途径中。

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PURPOSE: To determine the distribution of matrix metalloproteinase-1 (MMP-1) in the uveoscleral outflow pathway and other anterior segment tissues of normal human eyes. METHODS: Normal human eyes were fixed in methacarn and sectioned and immunostained using a specific polyclonal antibody to MMP-1. Immunoreactivity was visualized using diaminobenzidine. To compare the staining intensity in various tissues, the mean optical density within the ciliary body, mid-iris stroma, iris root, uveal trabecular meshwork, cornea, and sclera was determined using imaging densitometry. To determine the cellular distribution of MMP-1 in ciliary muscle, additional sections were double-immunostained using antibodies to MMP-1 and calponin. These sections were examined by confocal laser scanning microscopy. Specificity of the antibody to MMP-1 in ocular tissues was confirmed by western blot analysis with uveal tract homogenates. RESULTS: Moderate-to-strong MMP-1 immunoreactivity was observed in ciliary muscle, iris, sclera, corneal endothelium, and ciliary nonpigmented epithelium. Lighter immunoreactivity was observed in corneal epithelium, blood vessels, trabecular meshwork, Schlemm's canal, and associated collector channels. Confocal microscopy showed that ciliary muscle MMP-1 was primarily inside ciliary muscle cells. Densitometry showed that net optical density was approximately fivefold greater in ciliary muscle, iris root, and sclera than in trabecular meshwork. CONCLUSIONS: MMP-1 was prominently identified in regions of the anterior segment of normal human eyes associated with the uveoscleral outflow pathway and in the iris, corneal endothelium, and ciliary nonpigmented epithelium. These data support the hypothesis that MMP-1 activity is involved in regulating uveoscleral outflow facility.
机译:目的:确定基质金属蛋白酶-1(MMP-1)在正常人眼的葡萄膜巩膜流出途径和其他前节组织中的分布。方法:将正常人的眼睛固定在美沙康中,切片并使用针对MMP-1的特异性多克隆抗体进行免疫染色。使用二氨基联苯胺显示免疫反应性。为了比较各种组织的染色强度,使用成像光密度法确定了睫状体,中虹膜基质,虹膜根,葡萄膜小梁网,角膜和巩膜的平均光密度。为了确定MMP-1在睫状肌中的细胞分布,使用MMP-1和钙蛋白的抗体对其他切片进行双重免疫染色。通过共聚焦激光扫描显微镜检查这些切片。通过葡萄膜匀浆的蛋白质印迹分析证实了针对眼组织中MMP-1的抗体特异性。结果:在睫状肌,虹膜,巩膜,角膜内皮和睫状非色素上皮中观察到中等至强MMP-1免疫反应。在角膜上皮,血管,小梁网,Schlemm管和相关的收集器通道中观察到较轻的免疫反应性。共聚焦显微镜显示,睫状肌MMP-1主要位于睫状肌细胞内部。密度测定法显示,睫状肌,虹膜根和巩膜的净光密度比小梁网高约五倍。结论:MMP-1在正常人眼前段与葡萄膜巩膜流出通路相关的区域以及虹膜,角膜内皮和睫状非色素上皮细胞中得到了明显的鉴定。这些数据支持MMP-1活性参与调节葡萄膜巩膜流出设施的假设。

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