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Formation of lipofuscin-like material in the RPE Cell by different components of rod outer segments

机译:杆外节段的不同成分在RPE细胞中形成脂褐素样物质

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摘要

The mechanisms that control the natural rate of lipofuscin accumulation in the retinal pigment epithelial (RPE) cell and its stability over time are not well understood. Similarly, the contributions of retinoids, phospholipids and oxidation to the rate of accumulation of lipofuscin are uncertain. The experiments in this study were conducted to explore the individual contribution of rod outer segments (ROS) components to lipofuscin formation and its accumulation and stability over time. During the period of 14 days incubation of ROS, lipofuscin-like autofluorescence (LLAF) determined at two wavelengths (530 and 585 nm) by fluorescence-activated cell sorting (FACS) was measured from RPE cells. The autofluorescence increased in an exponential manner with a strong linear component between days 1 and 7. The magnitude of the increase was larger in cells incubated with 4-hydroxynonenal (HNE-ROS) compared with cells incubated with either bleached or unbleached ROS, but with a different spectral profile. A small (10–15%) decrease in LLAF was observed after stopping the ROS feeding for 14 days. The phagocytosis rate of HNE-ROS was higher than that of either bleached or unbleached ROS during the first 24 h of supplementation. Among the different ROS components, the increase of LLAF was highest in cells incubated with all-trans-retinal. Surprisingly, incubation with 11-cis-retinal and 9-cis-retinal also resulted in strong LLAF increase, comparable to the increase induced by all-trans-retinal. Supplementation with liposomes containing phosphatidylethanolamine (22: 6-PE) and phosphatidylcholine (18:1-PC) also increased LLAF, while incubation with opsin had little effect. Cells incubated with retinoids demonstrated strong dose-dependence in LLAF increase, and the magnitude of the increase was 2–3 times higher at 585 nm compared to 530 nm, while cells incubated with liposomes showed little dose-dependence and similar increase at both wavelengths. Very little difference in LLAF was noted between cells incubated with either unbleached or bleached ROS under any conditions. In summary, results from this study suggest that supplementation with various ROS components can lead to an increase in LLAF, although the autofluorescence generated by the different classes of components has distinct spectral profiles, where the autofluorescence induced by retinoids results in a spectral profile closest to the one observed from human lipofuscin. Future fluorescence characterization of LLAF in vitro would benefit from an analysis of multiple wavelengths to better match the spectral characteristics of lipofuscin in vivo.
机译:控制脂蛋白在视网膜色素上皮(RPE)细胞中的自然积累速率及其随时间变化的稳定性的机制尚不清楚。同样,类维生素A,磷脂和氧化对脂褐素积累速率的贡献尚不确定。进行了这项研究中的实验,以探索杆外部片段(ROS)组分对脂褐素形成及其随时间的积累和稳定性的个别贡献。在ROS孵育14天的过程中,从RPE细胞中测量了通过荧光激活细胞分选(FACS)在两个波​​长(530和585 nm)处测定的脂褐素样自发荧光(LLAF)。在第1天到第7天之间,自体荧光以指数方式增加,并带有强线性成分。与用漂白或未漂白ROS孵育的细胞相比,用4-羟基壬烯醛(HNE-ROS)孵育的细胞的增加幅度更大。不同的光谱轮廓。在停止ROS喂食14天后,观察到LLAF的小幅下降(10-15%)。在补充的头24小时内,HNE-ROS的吞噬率高于漂白或未漂白的ROS。在不同的ROS成分中,LLAF的增加在全反式视网膜孵育的细胞中最高。出人意料的是,与11-顺-视网膜和9-顺-视网膜一起孵育还导致LLAF强烈增加,这与全反式视网膜引起的增加相当。补充含有磷脂酰乙醇胺(22:6-PE)和磷脂酰胆碱(18:1-PC)的脂质体,也会增加LLAF,而与视蛋白孵育几乎没有效果。与类视黄醇一起孵育的细胞在LLAF的增加中表现出强烈的剂量依赖性,并且在585 nm处的增加幅度是530 nm的2-3倍,而与脂质体一起孵育的细胞在两个波长下均显示出很小的剂量依赖性和相似的增加。在任何条件下,用未漂白或漂白的ROS孵育的细胞之间,LLAF的差异很小。总而言之,这项研究的结果表明,尽管不同类别的组分产生的自发荧光具有独特的光谱特征,但补充各种ROS成分可导致LLAF升高,其中类维生素A诱导的自发荧光导致最接近的光谱特征从人脂褐素中观察到的一种。未来LLAF的体外荧光表征将受益于多种波长的分析,以更好地匹配体内脂褐素的光谱特征。

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