人体和动物透镜的核磁共振和荧光研究。

Lens and eye toxicity research Pub Date : 1991-01-01
S Lerman
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引用次数: 0

摘要

我们的实验室已经证明了非侵入性生物物理方法在研究白内障发生方面的潜力。最初,这些研究涉及对切除的晶状体或晶状体物质进行体外光谱分析(紫外、荧光和磷光)。此外,我们对提取的晶状体进行了核磁共振脉冲弛豫研究,结果表明正常晶状体的T1和T2值与年龄相关。体外荧光和核磁共振数据为体内监测人类和动物晶状体提供了潜在的参数。然后,我们利用Scheimpflug相机开发了体内晶状体荧光密度成像技术,并且最近使用我们的磁共振成像(MRI)方法(使用特殊构造的小线圈)来测量体内适度结合的晶状体水隔区(T2)。这两种体内方法都与我们的体外数据相关联,它们证明了正常晶状体的年龄相关变化;-即-荧光强度逐渐增加,T2值变长。已开发的指数,使我们能够检测异常晶状体荧光和变化的适度结合晶状体水(T2)的正常值与每一个特定年龄组的十年。这两种非侵入性生物物理技术可以在活体透明晶状体中检测到白内障前的变化,比传统的裂隙灯方法发现任何类型的混浊都早几个月到几年。MRI技术可在20分钟内完成,晶状体荧光法需要4-6分钟;因此,它们提供了一种快速客观的活体晶状体状态的体内测量方法,以及一种评估抗白内障药物疗效的方法。
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NMR & fluorescence studies on human and animal lenses.

Our laboratory has demonstrated the potential of non-invasive biophysical methods in studying cataractogenesis. Initially these studies involved in vitro spectroscopic assays (UV, fluorescence and phosphorescence) on excised lenses or lens matter. In addition, we performed NMR pulse relaxation studies on extracted lenses which demonstrated an age-related increase in the T1 and T2 values of the normal lens. The in vitro fluorescence and NMR data suggested potential parameters for monitoring human and animal lenses in vivo. We then developed in vivo lens fluorescence densitography utilizing the Scheimpflug camera and have recently employed our Magnetic Resonance Imaging (MRI) method (using specially constructed small coils) to measure the moderately bound lens water compartment (T2) in vivo. Both of these in vivo methods correlate with our in vitro data and they demonstrate age-related changes in the normal lens; - i.e. - a progressive increase in fluorescence intensity and longer T2 values. Indices have been developed which permit us to detect abnormal lens fluorescence and changes in the moderately bound lens water (T2) compared with normal values for each specific age group by decade. These 2 non-invasive biophysical techniques can detect pre-cataractous changes in the living clear lens, months to years before any type of opacity becomes manifest with the conventional slit lamp method. The MRI technique can be performed in less than 20 minutes and the lens fluorescence method requires 4-6 minutes; thus they provide a rapid and objective in vivo measure of the status of the living lens as well as a method for evaluating anti-cataract drug efficacy.

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