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Light Fractionation increases the Efficacy of ALA-PDT but not of MAL-PDT What is the Role of (Vascular) Endothelial Cells?

机译:光分级提高了ALA-PDT的功效,但没有提高MAL-PDT的功效(血管)内皮细胞的作用是什么?

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Photodynamic therapy (PDT) using protoporpyrin IX (PpIX) precursors like 5-aminolevulinic acid (ALA) or methyl-aminolevulinate (MAL) has shown to be effective in the treatment of various skin diseases. Using ALA we have shown in numerous studies a significantly improved efficacy by applying light fractionation with a long dark interval. In contrast, in the hairless mouse model, the PDT efficacy using MAL is unaffected by adopting this approach. More acute edema is found after ALA-PDT suggesting a difference in response of endothelial cells to PDT.To investigate the role of endothelial cells, cryo-sections of hairless mouse skin after 4 hours of topical MAL or ALA application were stained with a fluorescent endothelial cell marker (CD31). Co-localization of this marker with the PpIX fluorescence was performed using the spectral imaging function of the confocal microscope. We have also used intra-vital confocal microscopy to image the PpIX fluorescence distribution in correlation with the vasculature of live mouse skin.Our results show PpIX fluorescence at depth in cryo-sections of mouse skin after 4 hours of topical application. Co-localization has shown to be difficult due to the changes in tissue organization caused by the staining procedure. As expected we found high PpIX fluorescence levels in the epidermis after both MAL and ALA application using intra-vital microscopy. After ALA application more PpIX fluorescence was found deep in the dermal layer of the skin than after MAL. Furthermore we detected localized fluorescence in unidentified structures that could not be correlated to blood vessels or nerves.
机译:使用原卟啉IX(PpIX)前体(如5-氨基乙酰丙酸(ALA)或氨基-氨基乙酰丙酸甲酯(MAL))进行光动力疗法(PDT)已显示出可有效治疗各种皮肤疾病。使用ALA,我们在大量研究中显示了通过以较长的暗间隔进行光分馏,可以显着提高疗效。相反,在无毛小鼠模型中,采用这种方法不会影响使用MAL的PDT功效。在ALA-PDT后发现更多急性水肿,提示内皮细胞对PDT的反应有所不同。 为研究内皮细胞的作用,局部应用MAL或ALA 4小时后,无毛小鼠皮肤的冷冻切片用荧光内皮细胞标记物(CD31)染色。使用共聚焦显微镜的光谱成像功能将这种标记与PpIX荧光共定位。我们还使用了活体内共聚焦显微镜对与活小鼠皮肤的脉管系统相关的PpIX荧光分布进行了成像。 我们的结果显示,局部应用4小时后,小鼠皮肤冷冻切片的深处PpIX荧光很深。由于染色程序导致组织组织的变化,共定位已显示出困难。如所预期的,我们使用活体显微镜在MAL和ALA施用后在表皮中发现了高PpIX荧光水平。施用ALA后,与MAL后相比,在皮肤真皮层深处发现更多的PpIX荧光。此外,我们在无法识别的结构中检测到了无法与血管或神经相关的局部荧光。

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