首页> 外文期刊>Cornea >In vivo confocal microscopic evaluation of langerhans cell density and distribution in the corneal epithelium of healthy volunteers and contact lens wearers.
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In vivo confocal microscopic evaluation of langerhans cell density and distribution in the corneal epithelium of healthy volunteers and contact lens wearers.

机译:体内共聚焦显微镜评估健康志愿者和隐形眼镜佩戴者角膜上皮中的兰氏细胞密度和分布。

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PURPOSE: To examine and compare the density and distribution of Langerhans cells (LCs) in the corneal epithelium of healthy volunteers and contact lens wearers. METHODS: A total of 225 eyes of 130 healthy volunteers (age, 17-81 years) without history of ocular inflammation, trauma, or surgery and 98 eyes of 55 contact lens wearers (age, 13-76 years) were examined in vivo with the combination of the Heidelberg Retina Tomograph II and in-house-invented Rostock Cornea Module. RESULTS: In healthy volunteers, in vivo confocal microscopy revealed LCs in 31% of all volunteers, with 37 of these 43 volunteers presenting LCs both in the center and the periphery of the cornea with densities of 34 +/- 3 and 98 +/- 8 cells/mm, respectively. In the group of contact lens wearers, 55% of all corneas presented with LCs, and 11 of these 33 corneas revealed LCs at central and peripheral locations. Although LC densities were markedly higher in both the central (78 +/- 25 cells/mm) and the peripheral cornea (210 +/- 24 cells/mm) of contact lens wearers, the gradient of LC density from peripheral to central cornea was found almost identical in both groups. In the central cornea, LC density decreased with duration of contact lens wear. LCs were located at the depth of 35 to 60 microm (ie, the level of lower intermediate cells, basal cells, and subepithelial nervous plexus). LCs presented as either large cells bearing long processes or smaller cells lacking cell dendrites, most supposedly indicating mature and immature phenotype, respectively. CONCLUSIONS: In vivo confocal microscopy enables evaluation of LC density and distribution in corneal epithelium. LCs were found present both in the center and the periphery of the cornea without difference in distribution between healthy volunteers and contact lens wearers. However, contact lens wearers revealed almost twofold higher LC densities in both locations, implying chronic mechanical irritation of the cornea in response to the contact lens as foreign body. Taken together, analysis of LC using in vivo confocal microscopy provides helpful information for a better understanding of contact lens-disturbed ocular homeostasis.
机译:目的:检查和比较健康志愿者和隐形眼镜佩戴者角膜上皮中朗格汉斯细胞(LC)的密度和分布。方法:对130名健康的志愿者(年龄17-81岁)的225眼没有眼部炎症,外伤或手术史,对55名隐形眼镜佩戴者(13-76岁)的98眼进行了体内检查。海德堡Retina Tomograph II和内部发明的Rostock Cornea模块的组合。结果:在健康志愿者中,体内共聚焦显微镜检查显示所有参与者中有31%的LC,这43名志愿者中有37名在角膜中心和周边均出现LC,密度分别为34 +/- 3和98 +/-。分别为8格/毫米。在角膜接触镜配戴者组中,所有角膜中有55%出现LC,而这33个角膜中有11个在中央和周边位置出现了LC。尽管角膜接触镜佩戴者的中央角膜(78 +/- 25个/ mm)和周围角膜的LC密度均显着较高,但从周边角膜中央到中央角膜的LC密度梯度是在两组中发现几乎相同。在角膜中央,LC密度随着隐形眼镜佩戴时间的延长而降低。 LC位于35至60微米的深度(即较低的中间细胞,基底细胞和上皮下神经丛的水平)。 LC表现为具有长进程的大细胞或缺乏细胞树突的较小细胞,据推测分别指示成熟和未成熟的表型。结论:体内共聚焦显微镜能够评估LC密度和角膜上皮的分布。发现LC存在于角膜的中央和周边,而健康志愿者和隐形眼镜佩戴者之间的分布没有差异。然而,隐形眼镜佩戴者在两个位置上都显示出几乎两倍高的LC密度,这意味着响应于作为异物的隐形眼镜,对角膜的慢性机械刺激。综上所述,使用体内共聚焦显微镜对LC进行分析可提供有用的信息,有助于更好地了解隐形眼镜扰动的眼内稳态。

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