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Organization of junctional proteins in proliferating cat corneal endothelium during wound healing.

机译:伤口愈合过程中结缔组织蛋白在增殖性猫角膜内皮中的组织。

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PURPOSE: To evaluate for the first time cell junctional protein organization in proliferating corneal endothelial cells during in vivo wound healing. METHODS: A total of 16 cats (32 eyes) were used in this study. A single 3-mm diameter (n = 24) or 1- to 2-mm diameter (n = 8) scrape injury was created in the central corneal endothelium of each eye. Twenty-four, 48, 72 hours or 5 days after scrape injury, eyes were collected for in situ double- or triple-labeling with phalloidin, anti-ZO-1, alpha-catenin, beta-catenin, and MIB-1 (monoclonal antibody to Ki67, a marker for actively cycling cells) and were imaged using confocal laser microscopy. RESULTS: In 3-mm diameter injuries, endothelial cells completely resurfaced the wound 48 to 72 hours after scrape injury; smaller wounds resurfaced by 48 hours. Ki67 staining was negative 24 hours after scrape injury in all cases. Ki67-positive cells were observed in the central region of the wounds after 48 and 72 hours, and mitotic figures and pairs of postmitotic cells were observed. On day 5, Ki67-positive cells were rarely detected, and no mitotic figures were observed. In the wound area, a significant increase in cell area and a reduction in hexagonality were observed in cycling cells after 48 and 72 hours. Normal apical, pericellular staining of f-actin, ZO-1, alpha-catenin, and beta-catenin was partially maintained at all times during wound healing of small and large wounds. Double-labeling confirmed that these proteins were also present along the apical cell border in Ki67-positive cells. CONCLUSIONS: After in vivo scrape injury, proliferation is limited temporally and spatially to spreading endothelial cells within the wound. Cell junctional connections appear to be maintained in actively cycling cells during healing.
机译:目的:首次评估体内伤口愈合过程中角膜内皮细胞增殖的细胞连接蛋白组织。方法:本研究共使用16只猫(32只眼)。在每只眼睛的中央角膜内皮中产生了一个直径为3毫米(n = 24)或直径为1至2毫米(n = 8)的刮擦伤。刮擦伤后的24、48、72小时或5天,收集眼球以用鬼笔环肽,抗ZO-1,α-catenin,β-catenin和MIB-1(单克隆)原位进行双或三标记Ki67抗体(Ki67抗体,它是主动循环细胞的标志物),并使用共聚焦激光显微镜成像。结果:在3毫米直径的损伤中,内皮细胞在刮擦损伤后48至72小时完全重现了伤口。较小的伤口在48小时后重新出现。在所有情况下,刮擦后24小时Ki67染色均为阴性。在48小时和72小时后,在伤口的中央区域观察到Ki67阳性细胞,并且观察到有丝分裂图和成对的有丝分裂后细胞。在第5天,很少检测到Ki67阳性细胞,并且没有观察到有丝分裂图。在伤口区域,在48和72小时后,在循环细胞中观察到细胞面积显着增加,六角形减少。在小伤口和大伤口的愈合过程中,在任何时候都始终保持正常的根尖,细胞周围f-actin,ZO-1,α-catenin和β-catenin染色。双重标记证实了这些蛋白也出现在Ki67阳性细胞的顶端细胞边界。结论:体内刮擦损伤后,增殖在时间和空间上受到限制,只能在伤口内扩散内皮细胞。在愈合过程中,似乎在主动循环的细胞中维持了细胞连接连接。

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