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Characterizing the Effects of VPA VC and RCCS on Rabbit Keratocytes onto Decellularized Bovine Cornea

机译:表征VpaVC对兔角膜农村信用社在脱细胞牛角膜的影响和

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摘要

To investigate the morphological and growth characteristics of rabbit keratocytes when cultured on decellularized cornea under simulate microgravity (SMG) rotary cell culture system (RCCS) and static culture or in plastic culture supplemented with small molecules of valproic acid (VPA) and vitamin C (VC). Bovine corneas were firstly decellularized with Triton X-100 and NH4OH and through short-term freezing process. Then cell count kit-8 (CCK-8) and flow cytometry were used to test the effects of VPA and VC on the proliferation, cell cycle and apoptosis of rabbit keratocytes. Hematoxylin-eosin (H&E) staining and scanning electron microscopy (SEM) imaging showed that cells were eliminated in the decellularized bovine corneas. The proliferation of cultured keratocytes was promoted by VPA and VC in the cell proliferation assay. VPA and VC moderately decreased the number of apoptotic cells and obviously promoted cell-cycle entrance of keratocytes. Rabbit keratocytes in plastic displayed spindle shape and rare interconnected with or without VPA and VC. Cells revealed dendritic morphology and reticular cellular connections when cultured on the carriers of decellularized corneas supplemented with VPA and VC even in the presence of 10% fetal bovine serum (FBS). When cultured in RCCS supplemented with VPA, VC and 10% FBS, keratocytes displayed round shape with many prominences and were more prone to grow into the pores of carriers with aggregation. Reverse transcription-polymerase chain reaction (RT-PCR) analysis proved that the keratocytes cultured on decellularized bovine cornea under SMG with VPA and VC expressed keratocan and lumican. Keratocytes cultured on plastic expressed lumican but not keratocan. Immunofluorescence identification revealed that cells in all groups were positively immunostained for vimentin. Keratocytes on decellularized bovine cornea under SMG or in static culture were positively immunostained for keratocan and lumican. Thus, we reasonably made a conclusion that the combination of VPA, VC, RCCS and decellularized corneal carriers provide a good condition for keratocytes to well grow. Keratocytes can be manipulated to be aggregates or physiological morphological growth in vitro, which are important for the research of corneal stem cells and corneal tissue engineering.
机译:研究在模拟微重力(SMG)旋转细胞培养系统(RCCS)和静态培养或补充小分子丙戊酸(VPA)和维生素C(VC)的塑性培养下在脱细胞角膜上培养兔角膜细胞的形态和生长特征)。牛角膜首先通过Triton X-100和NH4OH并通过短期冷冻过程脱细胞。然后使用细胞计数试剂盒8(CCK-8)和流式细胞仪检测VPA和VC对兔角膜细胞增殖,细胞周期和凋亡的影响。苏木精-伊红(H&E)染色和扫描电子显微镜(SEM)成像显示,在脱细胞的牛角膜中细胞被清除。在细胞增殖测定中,VPA和VC促进了培养的角膜细胞的增殖。 VPA和VC适度减少了凋亡细胞的数量,并明显促进了角化细胞的细胞周期进入。塑料的兔角膜细胞呈纺锤形,很少与VPA和VC互连。当在添加有VPA和VC的脱细胞角膜载体上培养时,即使在10%胎牛血清(FBS)存在的情况下,细胞也显示出树突形态和网状细胞连接。当在补充有VPA,VC和10%FBS的RCCS中培养时,角质形成的细胞呈圆形,并具有许多突出的特征,并且更容易长成带有聚集体的载体孔。逆转录-聚合酶链反应(RT-PCR)分析证明,在SMG上用VPA和VC在脱细胞牛角膜上培养的角膜细胞表达了角蛋白聚糖和发光胶。在塑料上培养的角质形成细胞表达lumican,但不表达圆锥角蛋白。免疫荧光鉴定显示,所有组的细胞都对波形蛋白进行了阳性免疫染色。在SMG或静态培养条件下,去细胞牛角膜上的角质形成细胞对keratocan和lumican进行了阳性免疫染色。因此,我们合理地得出结论,VPA,VC,RCCS和脱细胞角膜载体的结合为角膜细胞的良好生长提供了良好条件。角质细胞可以在体外被操纵为聚集体或生理形态生长,这对于角膜干细胞和角膜组织工程的研究很重要。

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