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连续外植体培养为角膜内皮祖细胞的潜在位置和表型提供了新的见解。

Serial explant culture provides novel insights into the potential location and phenotype of corneal endothelial progenitor cells.

作者信息

Walshe Jennifer, Harkin Damien G

机构信息

Queensland Eye Institute, 140 Melbourne St, South Brisbane, QLD 4101, Australia.

Queensland Eye Institute, 140 Melbourne St, South Brisbane, QLD 4101, Australia; School of Biomedical Sciences, Queensland University of Technology, 2 George Street, Brisbane, Queensland 4001, Australia; Institute of Health and Biomedical Innovation, 60 Musk Avenue, Kelvin Grove, Queensland 4059, Australia.

出版信息

Exp Eye Res. 2014 Oct;127:9-13. doi: 10.1016/j.exer.2014.07.002. Epub 2014 Jul 14.

Abstract

The routine cultivation of human corneal endothelial cells, with the view to treating patients with endothelial dysfunction, remains a challenging task. While progress in this field has been buoyed by the proposed existence of progenitor cells for the corneal endothelium at the corneal limbus, strategies for exploiting this concept remain unclear. In the course of evaluating methods for growing corneal endothelial cells, we have noted a case where remarkable growth was achieved using a serial explant culture technique. Over the course of 7 months, a single explant of corneal endothelium, acquired from cadaveric human tissue, was sequentially seeded into 7 culture plates and on each occasion produced a confluent cell monolayer. Sample cultures were confirmed as endothelial in origin by positive staining for glypican-4. On each occasion, small cells, closest to the tissue explant, developed into a highly compact layer with an almost homogenous structure. This layer was resistant to removal with trypsin and produced continuous cell outgrowth during multiple culture periods. The small cells gave rise to larger cells with phase-bright cell boundaries and prominent immunostaining for both nestin and telomerase. Nestin and telomerase were also strongly expressed in small cells immediately adjacent to the wound site, following transfer of the explant to another culture plate. These findings are consistent with the theory that progenitor cells for the corneal endothelium reside within the limbus and provide new insights into expected expression patterns for nestin and telomerase within the differentiation pathway.

摘要

为了治疗内皮功能障碍患者而进行人角膜内皮细胞的常规培养仍然是一项具有挑战性的任务。尽管角膜缘存在角膜内皮祖细胞这一观点推动了该领域的进展,但利用这一概念的策略仍不明确。在评估角膜内皮细胞培养方法的过程中,我们注意到一个案例,即使用连续外植体培养技术实现了显著的细胞生长。在7个月的时间里,从尸体人类组织获取的单个角膜内皮外植体依次接种到7个培养皿中,每次都产生了汇合的细胞单层。通过对glypican - 4的阳性染色确认样本培养物来源于内皮细胞。每次,最靠近组织外植体的小细胞都会发育成具有几乎均匀结构的高度致密层。该层对胰蛋白酶具有抗性,并且在多个培养周期中产生连续的细胞生长。小细胞产生了具有明亮相细胞边界且对巢蛋白和端粒酶均有显著免疫染色的较大细胞。将外植体转移到另一个培养皿后,巢蛋白和端粒酶在紧邻伤口部位的小细胞中也强烈表达。这些发现与角膜内皮祖细胞存在于角膜缘的理论一致,并为巢蛋白和端粒酶在分化途径中的预期表达模式提供了新的见解。

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