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In vitro benzyl alcohol cytotoxicity: implications for intravitreal use of triamcinolone acetonide.

机译:体外苯甲醇的细胞毒性:对玻璃体内使用曲安奈德丙酮的影响。

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摘要

The aim of the study was to investigate the toxicity of benzyl alcohol (BA), the preservative in commercial triamcinolone acetonide (TA) suspensions, on retinal pigment epithelial (RPE) cells. Cultured RPE cells from a human cell line (ARPE-19) and from rabbits were exposed to the balanced salt solution (control) or BA (0.0225, 0.225, 0.9, 3 or 9mg/mL) for 5, 30, 60, or 120min. Morphological changes of RPE cells were evaluated by the trypan blue in situ staining. The proportions of dead cells were quantitatively measured by the trypan blue exclusion assay, and those of functional cells were assessed by a mitochondrial dehydrogenase assay. The mechanism of cytotoxicity was determined by the acridine orange/ethidium bromide staining and DNA laddering technique. Furthermore, ultrastructural changes were observed by transmission electron microscopy. The results showed that RPE cell damage was dose- and time-dependent. BA 0.225mg/mL, the clinically relevant concentration in TA following intravitreal injection, caused ultrastructural damage and impaired human RPE cell function at 2h; but BA 0.0225mg/mL did not. BA 9.0mg/mL, the concentration in commercial TA suspensions, was toxic within 5min on each assay for both human and rabbit RPE cells. The major mechanism of cell death was necrosis. In conclusion, BA in commercial TA suspensions injected intravitreally (0.225-9mg/mL) can damage RPE cells. Our in vitro study on benzyl alcohol cytotoxicity has significant clinical implications for intravitreal use of TA. We suggest that, before a commercial TA solution is used intravitreally, the vehicle should be removed to prevent damaging the RPE layer, particularly during macular hole surgery. Commercial development of a preservative-free TA suspension for intraocular use is urged.
机译:该研究的目的是研究商用曲安奈德丙酮(TA)悬浮液中的防腐剂苄醇(BA)对视网膜色素上皮(RPE)细胞的毒性。将来自人细胞系(ARPE-19)和兔子的RPE细胞暴露于平衡盐溶液(对照)或BA(0.0225、0.225、0.9、3或9mg / mL)中5、30、60或120min 。通过锥虫蓝原位染色评价RPE细胞的形态变化。通过台盼蓝排除试验定量测定死细胞的比例,通过线粒体脱氢酶测定评价功能细胞的比例。通过toxic啶橙/溴化乙锭染色和DNA标记技术确定了细胞毒性的机制。此外,通过透射电子显微镜观察到超微结构变化。结果表明,RPE细胞损伤是剂量和时间依赖性的。 BA 0.225mg / mL,玻璃体内注射后TA中的临床相关浓度,在2h时引起超微结构损伤和人类RPE细胞功能受损;但是BA 0.0225mg / mL没有。 BA 9.0mg / mL(市售TA悬浮液中的浓度)在每次测定中均在5分钟内对人和兔RPE细胞有毒。细胞死亡的主要机制是坏死。总之,玻璃体内注射的商业TA悬浮液中的BA(0.225-9mg / mL)可以损伤RPE细胞。我们对苯甲醇的细胞毒性的体外研究对玻璃体内使用TA具有重要的临床意义。我们建议,在玻璃体内使用商业化TA解决方案之前,应去除媒介物以防止损坏RPE层,尤其是在黄斑裂孔手术期间。敦促用于眼内使用的无防腐剂TA悬浮液的商业开发。

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