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[冷冻保存后器官培养中角膜上皮的形态学变化]

[Morphologic changes of corneal epithelium in organ culture after cryopreservation].

作者信息

Hagenah M, Böhnke M

机构信息

Universitäts-Augenklinik Hamburg.

出版信息

Ophthalmologe. 1993 Dec;90(6):679-82.

PMID:8124032
Abstract

Previous experimental studies concerning morphological changes of corneal endothelium after cryopreservation have been performed directly or within hours after thawing. The purpose of this study was to investigate morphological alterations of corneal endothelium up to 1 week after thawing in organ culture. We evaluated (1) pig corneas that were cryopreserved within 4 h of death, (2) pig corneas that had been stored in cryopreservation medium at 31 degrees C for 4 h before cryopreservation, and (3) as a control, corneas that were preserved in organ culture until the specific time of evaluation. Corneas were frozen to -196 degrees C in an automated freezing chamber in a cryopreservation medium containing chondroitin sulfate. Morphologic evaluation after trypan blue and alizarin red staining was performed after 1 day and after 1 week of organ culture preservation after thawing. One day after thawing, computer-assisted morphometric analysis of endothelial cell density and necrotic areas revealed endothelial cell loss of 25.7% in group 1 (8% necrosis), 48.7% in group 2 (17.4% necrosis) and 0% in group 3 (0% necrosis) compared to freshly dissected corneas. After 1 week, endothelial cell density had decreased by another 29% in groups 1 and 2 and by 11% in group 3 compared to results 1 day after thawing. However, necrotic areas could no longer be detected in any of the groups. We conclude that the highest decrease in endothelial cell density can be expected within 1 day after thawing. Further cell loss seems to be due to non-mitotic wound healing resulting in a confluent endothelial monolayer.

摘要

以往关于冷冻保存后角膜内皮形态变化的实验研究都是在解冻后直接进行或在数小时内进行。本研究的目的是在器官培养中研究解冻后长达1周的角膜内皮形态改变。我们评估了:(1)死亡后4小时内进行冷冻保存的猪角膜;(2)在冷冻保存前于31℃的冷冻保存培养基中储存4小时的猪角膜;以及(3)作为对照,在器官培养中保存至特定评估时间的角膜。角膜在含有硫酸软骨素的冷冻保存培养基中于自动冷冻室中冷冻至-196℃。在解冻后的器官培养保存1天和1周后,进行台盼蓝和茜素红染色后的形态学评估。解冻后1天,计算机辅助的内皮细胞密度和坏死区域形态计量分析显示,与新鲜解剖的角膜相比,第1组内皮细胞损失25.7%(坏死8%),第2组为48.7%(坏死17.4%),第3组为0%(坏死0%)。1周后,与解冻后1天的结果相比,第1组和第2组的内皮细胞密度又下降了29%,第3组下降了11%。然而,在任何一组中都不再能检测到坏死区域。我们得出结论,解冻后1天内内皮细胞密度的下降幅度最大。进一步的细胞损失似乎是由于非有丝分裂性伤口愈合导致内皮单层融合。

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1
[Morphologic changes of corneal epithelium in organ culture after cryopreservation].[冷冻保存后器官培养中角膜上皮的形态学变化]
Ophthalmologe. 1993 Dec;90(6):679-82.
2
[Effect of postmortem time on survival of corneal endothelium after cryopreservation].
Fortschr Ophthalmol. 1991;88(4):374-6.
3
[Freeze preservation of swine corneas with combinations of intra- and extracellular cryoprotective agents].[使用细胞内和细胞外冷冻保护剂组合对猪角膜进行冷冻保存]
Ophthalmologe. 1992 Dec;89(6):519-23.
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Klin Monbl Augenheilkd. 1996 Feb;208(2):107-11. doi: 10.1055/s-2008-1035179.
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Corneal cryopreservation with chondroitin sulfate.硫酸软骨素用于角膜冷冻保存。
Cryobiology. 1993 Aug;30(4):396-406. doi: 10.1006/cryo.1993.1039.
6
[Application of experimental findings of cryopreservation of animal tissue to results of cryopreservation of human tissue].[动物组织冷冻保存的实验结果在人体组织冷冻保存结果中的应用]
Fortschr Ophthalmol. 1990;87(2):218-20.
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Latent endothelial cell damage after experimental corneal cryopreservation.实验性角膜冷冻保存后的潜在内皮细胞损伤
Graefes Arch Clin Exp Ophthalmol. 1993 Sep;231(9):529-32. doi: 10.1007/BF00921118.
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[Experimental studies of the correlation of morphologic endothelial cell findings and endothelial pump function].
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Experimental corneal cryopreservation: impact of postmortem time on corneal endothelial cell survival.实验性角膜冷冻保存:死后时间对角膜内皮细胞存活的影响。
Ophthalmic Res. 1993;25(4):210-5. doi: 10.1159/000267315.
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[Cryopreservation of porcine corneas with chondroitin sulfate].[用硫酸软骨素对猪角膜进行冷冻保存]
Klin Monbl Augenheilkd. 1987 Oct;191(4):283-6. doi: 10.1055/s-2008-1050510.