用于保存角膜组织的合成介质，以备进行内皮角膜移植术和内皮细胞培养。

Synthetic media for preservation of corneal tissues deemed for endothelial keratoplasty and endothelial cell culture.

机构信息

Institute of Ophthalmology, University College London, London, UK.

International Center for Ocular Physiopathology, Fondazione Banca degli Occhi del Veneto Onlus, Venice, Italy.

出版信息

Acta Ophthalmol. 2021 May;99(3):314-325. doi: 10.1111/aos.14583. Epub 2020 Sep 10.

DOI:10.1111/aos.14583

PMID:32914554

Abstract

PURPOSE

To compare the difference between various endothelial graft preparation methods and endothelial cell culture from tissues that are preserved in serum-based and synthetic medium.

METHODS

In a randomized masked study, the tissues (n = 64) were preserved in Cornea Max (serum-based) and Cornea Syn (synthetic) series for 36 days at their respective preservation conditions. Following organ culture, corneal tissues (n = 48) were used to prepareDescemet stripping automated endothelial keratoplasty (DSAEK), preloaded ultra-thin (UT) -DSAEK, prestripped Descemet membrane endothelial keratoplasty (DMEK), free-floating DMEK, and preloaded DMEK with endothelium inward and outward grafts. These tissues were preserved for another 4days at room temperature in dextran supplemented media following which they were subjected to trypan blue, alizarin red, live/dead and Zonula Occludens-1 (ZO-1) staining. A separate set of tissues (n = 16) from both the series was used for human corneal endothelial cell (HCEnC) culture. At confluence, the proliferation and cell doubling rate was calculated and the cultured cells were subjected to live/dead, ZO-1, 2A12 and Ki-67 staining. Mann-Whitney test was performed with p < 0.05 deemed statistically significant.

RESULTS

After preparation and preservation of the tissues for endothelial keratoplasty, alizarin red showed standard endothelial morphology from both the groups. Endothelial cell loss, hexagonality and uncovered areas did not show statistically significant differences (p > 0.05) between both groups. For HCEnC, cell doubling rate was 4.7 days (p > 0.05). All the antibodies were expressed in both the groups. Hexagonality, polymorphism, cell area, viable/dead cells and Ki-67 positivity were not statistically significant (p > 0.05).

CONCLUSIONS

Complete synthetic organ culture series is safe and advantageous for carrying out advanced endothelial keratoplasty graft preparation procedures and for HCEnC culture as it is free from animal or animal-derived products.

摘要

目的

比较不同内皮移植物制备方法和在含血清和合成培养基中保存的组织培养内皮细胞之间的差异。

方法

在一项随机、双盲研究中，将组织（n=64）分别保存在 Cornea Max（含血清）和 Cornea Syn（合成）系列中，在各自的保存条件下保存 36 天。器官培养后，用角膜组织（n=48）制备 Descemet 撕囊自动化内皮角膜移植术（DSAEK）、预装超薄（UT）-DSAEK、预撕囊 Descemet 膜内皮角膜移植术（DMEK）、游离 DMEK 和内置和外置移植物的预装 DMEK。这些组织在室温下用葡聚糖补充培养基再保存 4 天，然后进行台盼蓝、茜素红、活/死和紧密连接蛋白-1（ZO-1）染色。从两个系列中各取一组组织（n=16）用于人角膜内皮细胞（HCEnC）培养。当细胞达到汇合时，计算细胞增殖和倍增率，并对培养的细胞进行活/死、ZO-1、2A12 和 Ki-67 染色。p<0.05 被认为具有统计学意义，采用曼-惠特尼检验。

结果

在进行内皮角膜移植术的组织准备和保存后，两组的茜素红均显示出标准的内皮形态。内皮细胞丢失、六边形和未覆盖面积在两组之间无统计学显著差异（p>0.05）。对于 HCEnC，细胞倍增率为 4.7 天（p>0.05）。两组均表达所有抗体。六边形、多态性、细胞面积、活/死细胞和 Ki-67 阳性率无统计学差异（p>0.05）。