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鼠角膜树突状细胞的荧光活体显微镜检查。

Epifluorescence intravital microscopy of murine corneal dendritic cells.

机构信息

Departments of Ophthalmology, Cell and Developmental Biology, Oregon Health and Science University, Portland, Oregon, USA.

出版信息

Invest Ophthalmol Vis Sci. 2010 Apr;51(4):2101-8. doi: 10.1167/iovs.08-2213. Epub 2009 Dec 10.

DOI:10.1167/iovs.08-2213
PMID:20007837
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2868401/
Abstract

Purpose. Dendritic cells (DCs) are antigen-presenting cells vital for initiating immune responses. In this study the authors examined the in vivo migratory capability of resident corneal DCs to various stimuli. Methods. The authors used mice expressing enhanced yellow fluorescent protein (eYFP) under control of the CD11c promoter to visualize corneal DCs. To assess the distribution and mobility of DCs, normal corneas were imaged in vivo and ex vivo with fluorescence microscopy. Intravital microscopy was used to examine the responses of resident central and peripheral corneal DCs to silver nitrate injury, lipopolysaccharide, microspheres, and tumor necrosis factor (TNF-alpha). In some experiments, TNF-alpha injection was used to first induce centripetal migration of DCs to the central cornea, which was subsequently reinjected with microspheres. Results. In normal corneas, DCs were sparsely distributed centrally and were denser in the periphery, with epithelial-level DCs extending into the epithelium. Videomicroscopy showed that though cell processes were in continuous movement, cells generally did not migrate. Within the first 6 hours after stimulation, neither central nor peripheral corneal DCs exhibited significant lateral migration, but central corneal DCs assumed extreme morphologic changes. An increased number of DCs in the TNF-alpha-stimulated central cornea were responsive to subsequent microsphere injection by adopting a migratory behavior, but not with increased speed. Conclusions. In vivo imaging reveals minimal lateral migration of corneal DCs after various stimuli. In contrast, DCs within the central cornea after initial TNF-alpha injection are more likely to respond to a secondary insult with lateral migration.

摘要

目的

树突状细胞(DCs)是启动免疫反应所必需的抗原呈递细胞。本研究作者研究了常驻角膜 DCs 对各种刺激物的体内迁移能力。

方法

作者使用表达增强型黄色荧光蛋白(eYFP)的小鼠,其表达受 CD11c 启动子的控制,以可视化角膜 DCs。为了评估 DCs 的分布和迁移能力,作者使用荧光显微镜对正常角膜进行体内和体外成像。使用活体显微镜检查来研究常驻中央和周边角膜 DCs 对硝酸银损伤、脂多糖、微球和肿瘤坏死因子(TNF-α)的反应。在一些实验中,使用 TNF-α 注射首先诱导 DCs 向中央角膜的向心迁移,然后用微球对其进行再注射。

结果

在正常角膜中,DCs 稀疏地分布在中央,在周边更密集,上皮层的 DCs 延伸到上皮层。视频显微镜显示,尽管细胞突起处于连续运动中,但细胞通常不会迁移。在刺激后 6 小时内,中央和周边角膜 DCs 均未表现出明显的侧向迁移,但中央角膜 DCs 呈现出极端的形态变化。TNF-α 刺激的中央角膜中更多的 DCs 对随后的微球注射表现出迁移行为的反应,但速度没有增加。

结论

体内成像显示,各种刺激后角膜 DCs 的侧向迁移很少。相比之下,初始 TNF-α 注射后的中央角膜中的 DCs 更有可能通过侧向迁移对二次损伤作出反应。

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