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Optimization of in vivo confocal autofluorescence imaging of the ocular fundus in mice and its application to models of human retinal degeneration.

机译:小鼠眼底体内共聚焦自发荧光成像的优化及其在人视网膜变性模型中的应用。

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摘要

PURPOSE: To investigate the feasibility and to identify sources of experimental variability of quantitative and qualitative fundus autofluorescence (AF) assessment in mice. METHODS: Blue (488 nm) and near-infrared (790 nm) fundus AF imaging was performed in various mouse strains and disease models (129S2, C57Bl/6, Abca4(-/-), C3H-Pde6b(rd1/rd1), Rho(-/-), and BALB/c mice) using a commercially available scanning laser ophthalmoscope. Gray-level analysis was used to explore factors influencing fundus AF measurements. RESULTS: A contact lens avoided cataract development and resulted in consistent fundus AF recordings. Fundus illumination and magnification were sensitive to changes of the camera position. Standardized adjustment of the recorded confocal plane and consideration of the pupil area allowed reproducible recording of fundus AF from the retinal pigment epithelium with an intersession coefficient of repeatability of ±22%. Photopigment bleaching occurred during the first 1.5 seconds of exposure to 488 nm blue light (∼10 mW/cm(2)), resulting in an increase of fundus AF. In addition, there was a slight decrease in fundus AF during prolonged blue light exposure. Fundus AF at 488 nm was low in animals with an absence of a normal visual cycle, and high in BALB/c and Abca4(-/-) mice. Degenerative alterations in Pde6b(rd1/rd1) and Rho(-/-) were reminiscent of findings in human retinal disease. CONCLUSIONS: Investigation of retinal phenotypes in mice is possible in vivo using standardized fundus AF imaging. Correlation with postmortem analysis is likely to lead to further understanding of human disease phenotypes and of retinal degenerations in general. Fundus AF imaging may be useful as an outcome measure in preclinical trials, such as for monitoring effects aimed at lowering lipofuscin accumulation in the retinal pigment epithelium.
机译:目的:探讨可行性和鉴定小鼠定量和定性眼底自发荧光(AF)评估的实验变异性来源。方法:在各种小鼠品系和疾病模型(129S2,C57Bl / 6,Abca4(-/-),C3H-Pde6b(rd1 / rd1),小鼠和小鼠)中进行了蓝色(488 nm)和近红外(790 nm)眼底AF成像Rho(-/-)和BALB / c小鼠)使用市售的扫描激光检眼镜。灰度分析用于探索影响眼底房颤测量的因素。结果:隐形眼镜避免了白内障的发展,并导致一致的眼底房颤记录。眼底的照明和放大倍数对摄像机位置的变化很敏感。通过对记录的共焦平面进行标准化调整并考虑瞳孔面积,可以从视网膜色素上皮中再现性记录眼底房颤,其间期重复性为±22%。在暴露于488 nm蓝光(〜10 mW / cm(2))的前1.5秒内,发生了光色素的漂白,导致眼底房颤的增加。此外,长时间的蓝光暴露会使眼底房颤略有下降。在没有正常视觉周期的动物中,488 nm的眼底AF低,而在BALB / c和Abca4(-/-)小鼠中,眼底AF高。 Pde6b(rd1 / rd1)和Rho(-/-)的退化性改变让人联想到人类视网膜疾病的发现。结论:使用标准化眼底AF成像可以在体内研究小鼠的视网膜表型。与验尸分析的相关性可能会导致人们进一步了解人类疾病的表型和一般的视网膜变性。眼底AF成像可能在临床前试验中用作结果测量,例如用于监测旨在降低视网膜色素上皮中脂褐素积聚的效果。

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