玫瑰红光动力疗法对人角膜上皮细胞和基质细胞活力和增殖的体外评估

IF 0.8 4区 医学 Q4 OPHTHALMOLOGY Klinische Monatsblatter fur Augenheilkunde Pub Date : 2024-08-01 Epub Date: 2023-02-20 DOI:10.1055/a-2038-8899
Ning Chai, Tanja Stachon, Mahsa Nastaranpour, Zhen Li, Berthold Seitz, Myriam Ulrich, Achim Langenbucher, Nóra Szentmáry
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引用次数: 0

摘要

目的:研究玫瑰红光动力疗法(RB-PDT)对体外人角膜缘上皮干细胞(T-LSCs)、人角膜上皮细胞(HCE-T)、人角膜缘成纤维细胞(LFCs)以及人正常和角膜病成纤维细胞(HCFs 和 KC-HCFs)的活力和增殖的影响:本研究使用了 T-LSCs 和 HCE-T 细胞系。LFCs 从健康的供体角膜缘(n = 5)中分离出来,HCFs 从健康的人类供体角膜(n = 5)中分离出来,KC-HCFs 从角膜炎患者的穿透性角膜移植(n = 5)中分离出来。细胞培养后,使用浓度为 0.001% 的 RB 和波长为 565 nm、能量为 0.14 至 0.7 J/cm2 的照明进行 RB-PDT 试验。RB-PDT 24 小时后,用 XTT 和 BrdU 检测法评估细胞活力和增殖情况:结果:单独使用 RB 或光照不会改变任何细胞类型的细胞活力或增殖(p ≥ 0.1)。然而,在 RB-PDT 之后,HCFs 的存活率从 0.17 J/cm2 的荧光量(p 2 T-LSCs 的荧光量(p 2 T-LSCs 的荧光量(p 2 HCFs 的荧光量(p 结论))显著下降:尽管 RB-PDT 似乎是一种安全有效的体内治疗方法,但其对角膜上皮细胞和基质细胞的剂量依赖性光毒性必须得到尊重。本研究中应用的数据和实验参数可为今后的研究提供可靠的参考。
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Assessment of Rose Bengal Photodynamic Therapy on Viability and Proliferation of Human Keratolimbal Epithelial and Stromal Cells In Vitro.

Purpose: To investigate the effect of Rose Bengal photodynamic therapy (RB-PDT) on viability and proliferation of human limbal epithelial stem cells (T-LSCs), human corneal epithelial cells (HCE-T), human limbal fibroblasts (LFCs), and human normal and keratoconus fibroblasts (HCFs and KC-HCFs) in vitro.

Methods: T-LSCs and HCE-T cell lines were used in this research. LFCs were isolated from healthy donor corneal limbi (n = 5), HCFs from healthy human donor corneas (n = 5), and KC-HCFs from penetrating keratoplasties of keratoconus patients (n = 5). After cell culture, RB-PDT was performed using 0.001% RB concentration and 565 nm wavelength illumination with 0.14 to 0.7 J/cm2 fluence. The XTT and the BrdU assays were used to assess cell viability and proliferation 24 h after RB-PDT.

Results: RB or illumination alone did not change cell viability or proliferation in any of the cell types (p ≥ 0.1). However, following RB-PDT, viability decreased significantly from 0.17 J/cm2 fluence in HCFs (p < 0.001) and KC-HCFs (p < 0.0001), and from 0.35 J/cm2 fluence in T-LSCs (p < 0.001), HCE-T (p < 0.05), and LFCs ((p < 0.0001). Cell proliferation decreased significantly from 0.14 J/cm2 fluence in T-LSCs (p < 0.0001), HCE-T (p < 0.05), and KC-HCFs (p < 0.001) and from 0.17 J/cm2 fluence in HCFs (p < 0.05). Regarding LFCs proliferation, no values could be determined by the BrdU assay.

Conclusions: Though RB-PDT seems to be a safe and effective treatment method in vivo, its dose-dependent phototoxicity on corneal epithelial and stromal cells has to be respected. The data and experimental parameters applied in this study may provide a reliable reference for future investigations.

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