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首页> 外文期刊>The journal of clinical investigation >In vivo imaging of the human eye using a 2-photon-excited fluorescence scanning laser ophthalmoscope
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In vivo imaging of the human eye using a 2-photon-excited fluorescence scanning laser ophthalmoscope

机译:使用2-光子激发荧光扫描激光眼球镜的人眼的体内成像

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Background Noninvasive assessment of metabolic processes that sustain regeneration of human retinal visual pigments (visual cycle) is essential to improve ophthalmic diagnostics and to accelerate development of new treatments to counter retinal diseases. Fluorescent vitamin A derivatives, which are the chemical intermediates of these processes, are highly sensitive to UV light; thus, safe analyses of these processes in humans are currently beyond the reach of even the most modern ocular imaging modalities. Methods We present a compact, 2-photon-excited fluorescence scanning laser ophthalmoscope and spectrally resolved images of the human retina based on 2-photon excitation (TPE) with near-infrared light. A custom Er:fiber laser with integrated pulse selection, along with intelligent postprocessing of data, enables excitation with low laser power and precise measurement of weak signals. Results We demonstrate spectrally resolved TPE fundus images of human subjects. Comparison of TPE data between human and mouse models of retinal diseases revealed similarity with mouse models that rapidly accumulate bisretinoid condensation products. Thus, visual cycle intermediates and toxic byproducts of this metabolic pathway can be measured and quantified by TPE imaging. Conclusion Our work establishes a TPE instrument and measurement method for noninvasive metabolic assessment of the human retina. This approach opens the possibility for monitoring eye diseases in the earliest stages before structural damage to the retina occurs. Funding NIH, Research to Prevent Blindness, Foundation for Polish Science, European Regional Development Fund, Polish National Agency for Academic Exchange, and Polish Ministry of Science and Higher Education.
机译:背景技术对人视网膜视力(视觉周期)再生的代谢过程的非侵入性评估对于改善眼科诊断并加速新治疗以抵抗视网膜疾病至关重要。荧光维生素是这些方法的化学中间体的衍生物对紫外光非常敏感;因此,人类中这些过程的安全分析目前超出了甚至最现代眼镜成像模式的覆盖范围。方法我们介绍了一种紧凑的2-光子激发的荧光扫描激光眼科,基于具有近红外光的2-光子激发(TPE)的人视网膜的光谱分辨图像。自定义ER:具有集成脉冲选择的光纤激光器,以及智能的数据后处理,可激发低激光功率和精确测量弱信号的精确测量。结果我们展示了人类受试者的光谱解析TPE眼底图像。视网膜疾病人和小鼠模型之间TPE数据的比较显示了快速积聚双滴水凝固产物的小鼠模型的相似性。因此,通过TPE成像可以测量和量化该代谢途径的视觉周期中间体和毒性副产物。结论我们的工作建立了一种TPE仪器和用于人视网膜的非侵入性代谢评估的测量方法。这种方法在结构损伤发生之前,打开了在最早的阶段监测眼部疾病的可能性。资助NIH,研究防止盲肠,波兰科科学基金会,欧洲区域发展基金,波兰国家学术交流机构,波兰科学和高等教育部。

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