首页> 外文期刊>Journal of cataract and refractive surgery >Corneal cell response after flap creation using a mechanical microkeratome or a 200 kHz femtosecond laser
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Corneal cell response after flap creation using a mechanical microkeratome or a 200 kHz femtosecond laser

机译:使用机械微型电机组或200 kHz Femtosecond激光器的皮瓣创建后角膜细胞反应

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摘要

Purpose: To compare the inflammatory cell response within the corneal flap interface created by a mechanical microkeratome and a femtosecond laser. Setting: Department of Ophthalmology, Ludwig-Maximilians-University, Munich, Germany. Design: Experimental in vitro study. Methods: Corneoscleral buttons of 12 enucleated human eyes not suitable for transplantation were put into organ culture. Corneal flaps were created using a 200 kHz femtosecond laser (Visumax) (femtosecond group) or a mechanical microkeratome (Amadeus) (microkeratome group). Flaps were not lifted after treatment. In 2 corneas, no treatment was performed (control group). Corneas were kept in organ culture for 12 hours thereafter. To evaluate cell-mediated immune reaction, immunofluorescent staining for leucocytes (cluster of differentiation 45) and specifically for dendritic cells (human leukocyte antigen-DR) was performed in every group. A terminal deoxynucleotidyl transferase dUTP nick end labeling (TUNEL) assay was used to determine apoptosis reaction. Results: The ratio of dendritic cells in the femtosecond group compared with the microkeratome group was 1.2 (P=.02), the ratio of leucocytes was 1.4 (P=.06), and the ratio of apoptotic cells was 1.0 (P=.59). There was no marked significant difference in the distribution of inflammatory cell reaction. The control group showed neither specific inflammatory reaction nor apoptosis. Conclusion: This in vitro series of human corneas showed similar inflammatory tissue reaction after femtosecond laser-assisted and microkeratome-assisted flap creation (P<.05). Financial Disclosure: No author has a financial or proprietary interest in any material or method mentioned.
机译:目的:比较由机械微型电机组和飞秒激光器产生的角膜翼片界面内的炎症细胞响应。环境:德国慕尼黑,Ludwig-Maximilians-University的眼科培训部。设计:实验体外研究。方法:未适用于移植的12个Enucleated人眼的CorneoScleral按钮被放入器官培养物中。使用200kHz Femtosecond激光(Visumax)(Femtosecond Group)或机械微型计算机(Amadeus)(Microkatome组)来创建角膜翼片。治疗后没有提升襟翼。在2个角膜中,未进行治疗(对照组)。此后在器官培养物中保持玉米物12小时。为了评估细胞介导的免疫反应,对白细胞的免疫荧光染色(分化45),特别是在每组中进行树突细胞(人白细胞抗原-Dr)。末端脱氧核苷酸转移酶DUTP裂解末端标记(TUNEL)测定法用于确定凋亡反应。结果:与微立体组比较的小树枝状细胞比率与微立体组比较为1.2(p = .02),白细胞的比例为1.4(p = .06),凋亡细胞的比例为1.0(p =。 59)。炎症细胞反应的分布没有显着的显着差异。对照组既不显示特异性炎症反应也没有细胞凋亡。结论:这种体外系列人体玉米体在飞秒激光辅助和微型电磁体辅助襟翼创建后的相似炎症组织反应(P <.05)。财务披露:没有作者对提到的任何材料或方法都有财务或专有权益。

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    Department of Ophthalmology Ludwig-Maximilians-University Munich Campus Innenstadt;

    Department of Ophthalmology Ludwig-Maximilians-University Munich Campus Innenstadt;

    Department of Ophthalmology Ludwig-Maximilians-University Munich Campus Innenstadt;

    Department of Ophthalmology Ludwig-Maximilians-University Munich Campus Innenstadt;

    Department of Ophthalmology Ludwig-Maximilians-University Munich Campus Innenstadt;

    Department of Ophthalmology Ludwig-Maximilians-University Munich Campus Innenstadt;

    Department of Ophthalmology Ludwig-Maximilians-University Munich Campus Innenstadt;

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  • 中图分类 眼科学;
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