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Challenges in improving cell density of tissue-engineered corneal endothelium

机译:改善组织工程角膜内皮细胞密度的挑战

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Introduction: Comeal endothelial dysfunctions cause blindness and are the main indications for allogeneic comeal transplantation. Limited availability of donor corneas has motivated the development of tissue-engineered posterior corneas from cultured corneal endothelial cells (CECs). However, expansion of CECs in vitro induces cell enlargement and results in the formation a monolayer with low endothelial cell density (ECD). Our objective was to increase the ECD over the minimum density of 2000 cells/mm~2 required by eye banks. Materiel and Method: CECs were isolated form eye bank corneas and cultured as described in Zhu & Joyce. Different approaches were tested in order to increase ECD: 1) Cells were seeded at increasing cell densities (375 to 12 000 cells/mm~2) then cultured for 9 days before analysis. 2) Cells were seeded at 6 000 cells/mm2 then immediately centrifuged (300 g), cultured for 9 days, then analysed. Controls consisted of omitting the centrifugation step. 3) Small cells were selected by centrifugation on a Ficoll density gradient (1.059 g/ml) or cell strainers (10 μm - 15 μm). Cell size was analysed using a Coulter counter. 4) Cells were seeded at 1 000 cells/mm2 on a tissue engineered stromal substitute. After 2 weeks of culture, the engineered tissue was released from its anchor, allowing for contraction of the tissue. Macroscopic pictures were used to calculate de % of contraction. Calculation of ECD was either performed by counting the number of nucleus (Hoechst staining) using Cellproftler software (n=4 pictures/condition) or by morphometric analysis of alizarin red-stained endothelia. Results and Discussion: 1) ECD increased with the augmentation of cell seeding density. At 375 cells/mm~2, the monolayer reached 500 cells/mm2 while at 6000 cells/mm~2, the monolayer was 1400 cells/mm~2. However, when seeded at 12000 cells/mm~2, CECs aggregated and failed to adhere to the culture plate. 2) Centrifugation slightly increased ECD of cells seeded at 6000 cells/mm2 from 1400 to 1750 cells/mm~2, still under the minimal density for grafting. 3) The two methods tested to select the smallest cells failed to separate the small from the bigger cells. The final size of the cells separated by the cell strainers were 11.5 μm and 12.8 μm for the 10 and 15 μm cell strainer respectively (controls = 16.0 μm), while CEC of high and low density had respectively 14.8 μm and 16.5 μm in diameter. 4) The presence of endothelial cells reduced the tissue sheet contraction from 40% without CECs to 30% with CECs. The monolayers of CECs did not form proper cell-cell junction preventing the identification of cell borders following alizarin red staining and therefore morphometric analysis. Conclusion: Centrifugation at the time of cell seeding was the most promising technique to increased ECD. A combination of multiple approaches could be necessary to reach an acceptable ECD. Future experiments should also be aimed at maintaining the small cell size during the in vitro expansion process, which would generate engineered endothelia of high ECD.
机译:简介:彗星内皮功能障碍会导致失明,并且是异体彗星移植的主要适应症。供体角膜的有限供应已激发了培养的角膜内皮细胞(CEC)的组织工程化后角膜的发展。但是,体外CEC的扩增会诱导细胞扩增,并形成具有低内皮细胞密度(ECD)的单层细胞。我们的目标是在眼库要求的最小密度2000细胞/ mm〜2的范围内增加ECD。材料和方法:CECs从眼角膜分离并按照Zhu&Joyce中所述进行培养。为了增加ECD,测试了不同的方法:1)以增加的细胞密度(375至12,000个细胞/ mm〜2)接种细胞,然后在分析前培养9天。 2)以6000个细胞/ mm 2接种细胞,然后立即离心(300g),培养9天,然后进行分析。对照包括省略离心步骤。 3)通过在Ficoll密度梯度(1.059 g / ml)或细胞过滤器(10μm-15μm)上离心选择小细胞。使用库尔特计数器分析细胞大小。 4)将细胞以1000个细胞/ mm 2接种在组织工程改造的基质替代物上。培养2周后,工程组织从其锚固件中释放出来,从而使组织收缩。宏观图片用于计算收缩率。通过使用Cellproftler软件(n = 4张图片/条件)对核数进行计数(Hoechst染色)或通过茜素红染色的内皮细胞的形态分析来进行ECD的计算。结果与讨论:1)ECD随着细胞接种密度的增加而增加。在375个/ mm 2下,单层达到500个/ mm 2,而在6000个/ mm 2下,单层为1400个/ mm 2。然而,当以12000个细胞/ mm〜2的密度接种时,CEC聚集并且不能粘附在培养板上。 2)离心处理使以6000细胞/ mm2接种的细胞的ECD从1400升高到1750细胞/ mm〜2,仍处于嫁接的最小密度下。 3)测试用来选择最小单元的两种方法未能将较小的单元与较大的单元区分开。对于10和15μm的细胞过滤器,由细胞过滤器分离的细胞的最终大小分别为11.5μm和12.8μm(对照= 16.0μm),而高密度和低密度CEC的直径分别为14.8μm和16.5μm。 4)内皮细胞的存在将组织片的收缩率从无CEC的40%降低为有CEC的30%。 CEC的单层不能形成适当的细胞-细胞连接,从而阻止了茜素红染色和形态计量学分析之后的细胞边界鉴定。结论:细胞接种时的离心分离是增加ECD的最有前途的技术。为了达到可接受的ECD,可能需要多种方法的组合。未来的实验还应旨在在体外扩增过程中维持较小的细胞大小,这将产生高ECD的工程化内皮细胞。

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