Lu Xiaoyan, Chen Dong, Liu Zhiping, Li Chaoyang, Liu Ying, Zhou Jin, Wan Pengxia, Mou Yong-gao, Wang Zhichong
State Key laboratory of Ophthalmology, Sun Yat-sen University, Guangzhou, PR China.
Mol Vis. 2010 Apr 8;16:611-22. doi: 10.1167/2.7.611.
To determine whether mouse embryonic stem cell conditioned medium (ESC-CM) increases the proliferative capacity of human corneal endothelial cells (HCECs) in vitro.
Primary cultures of HCECs were established from explants of the endothelial cell layer, including the Descemet's membrane. Cells were cultured in human corneal endothelium medium (CEM) containing 25% ESC-CM for the experimental group and CEM alone for the control group. Phase-contrast microscopy and reverse-transcription polymerase chain reaction (RT-PCR) were used to identify HCECs. The eruption time and HCEC morphology were observed under phase-contrast microscopy. We detected the protein expression of zona occludens protein-1 (ZO-1; a tight junction protein) and the Na(+)-K(+)-ATPase by western blot analysis and immunocytochemistry. The mRNA expression of the Na(+)-K(+)-ATPase, voltage-dependent anion channel 3 (VDAC3), solute carrier family 4, sodium bicarbonate cotransporter member 4 (SLC4A4), and chloride channel protein 3 (CLCN3) were detected by RT-PCR. To explore the proliferation capacity of HCECs, the colony forming efficiency (CFE) was determined by Giemsa staining and the cellular proliferation marker of Ki-67 protein (Ki-67) positive cells were detected by immunocytochemistry and flow cytometry. Progression of the cell cycle and apoptosis were analyzed by flow cytometry. Negative regulation of the cell cycle, as measured by cyclin-dependent kinase inhibitor p21 (p21) levels, was detected by western blot analysis and immunocytochemistry.
In primary culture, HCECs in the 25%ESC-CM group erupted with polygonal appearance on day 2, while those in the CEM group erupted with slightly larger cells on day 3-4. HCECs in the 25%ESC-CM group could be subcultured until passage 6 without enlargement of cell volume, while those in the CEM group were enlarged and lost their polygonal appearance by passage 2. HCECs in both the 25%ESC-CM and CEM groups expressed ZO-1, Na(+)-K(+)-ATPase, VDAC3, SLC4A4, and CLCN3. The number of Ki67 positive cells, CFE, and percentage of cells entering the S and G(2) phases were higher in the 25%ESC-CM group than in the CEM group. The number of apoptotic cells and p21 protein expression both decreased in the 25%ESC-CM group.
Use of 25%ESC-CM significantly increased the number of proliferating cells. These effects may be achieved through inhibition of p21 expression and apoptosis. These results suggested that 25%ESC-CM may be a new tool for cultivating HCECs for transplantation.
确定小鼠胚胎干细胞条件培养基(ESC-CM)是否能在体外提高人角膜内皮细胞(HCECs)的增殖能力。
从包括Descemet膜在内的内皮细胞层外植体建立HCECs原代培养物。实验组细胞在含25% ESC-CM的人角膜内皮培养基(CEM)中培养,对照组细胞仅在CEM中培养。采用相差显微镜和逆转录聚合酶链反应(RT-PCR)鉴定HCECs。在相差显微镜下观察细胞出现时间和HCECs形态。通过蛋白质印迹分析和免疫细胞化学检测紧密连接蛋白-1(ZO-1)和钠钾ATP酶的蛋白表达。通过RT-PCR检测钠钾ATP酶、电压依赖性阴离子通道3(VDAC3)、溶质载体家族4、碳酸氢钠共转运体成员4(SLC4A4)和氯通道蛋白3(CLCN3)的mRNA表达。为探究HCECs的增殖能力,通过吉姆萨染色测定集落形成效率(CFE),并通过免疫细胞化学和流式细胞术检测细胞增殖标志物Ki-67蛋白(Ki-67)阳性细胞。通过流式细胞术分析细胞周期进程和细胞凋亡。通过蛋白质印迹分析和免疫细胞化学检测细胞周期负调控因子细胞周期蛋白依赖性激酶抑制剂p21(p21)的水平。
在原代培养中,25% ESC-CM组的HCECs在第2天呈多边形出现,而CEM组的细胞在第3 - 4天出现且细胞稍大。25% ESC-CM组的HCECs可传代至第6代而细胞体积无增大,而CEM组的细胞在传代至第2代时体积增大且失去多边形外观。25% ESC-CM组和CEM组的HCECs均表达ZO-1、钠钾ATP酶、VDAC3、SLC4A4和CLCN3。25% ESC-CM组的Ki67阳性细胞数量、CFE以及进入S期和G2期的细胞百分比均高于CEM组。25% ESC-CM组的凋亡细胞数量和p21蛋白表达均降低。
使用25% ESC-CM可显著增加增殖细胞数量。这些作用可能通过抑制p21表达和细胞凋亡来实现。这些结果表明,25% ESC-CM可能是一种用于培养用于移植的HCECs的新工具。
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