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促红细胞生成素对大鼠视网膜神经元轴突生长的促进作用及保护作用

Promotion of neurite outgrowth and protective effect of erythropoietin on the retinal neurons of rats.

作者信息

Zhong Yisheng, Yao Huiping, Deng Lianfu, Cheng Yu, Zhou Xiaoqing

机构信息

Department of Ophthalmology, Ruijin Hospital Affiliated Shanghai Jiaotong University, 197 Ruijin No.2 Road, 200025, Shanghai, People's Republic of China.

出版信息

Graefes Arch Clin Exp Ophthalmol. 2007 Dec;245(12):1859-67. doi: 10.1007/s00417-007-0671-9. Epub 2007 Sep 9.

Abstract

OBJECTIVE

To clarify the effect of erythropoietin (EPO) on neurite outgrowth of the cultured retinal neurocytes, and investigate whether EPO might potentially be beneficial in protecting cultured retinal neurocytes suffering from glutamate-induced cytotoxity.

METHODS

After the retinal neurocytes were cultured for 48 hours, the culture media was replaced with serum-free media, and the cultured retinal cells were exposed to 1.0 U/ml, 3.0 U/ml and 6.0 U/ml EPO for another 48 hours; then the cells were stained with Sudan Black B, and the neurite outgrowth of those cells were evaluated by an image-analysis system. After the retinal neurocytes were cultured for 48 hours, the cells were cultured in serum-free media containing 5 mM or 10 mM glutamate, and the cells were incubated in the presence or absence of Epo (1.0 U/ml, 3.0 U/ml, 6.0 U/ml respectively) for another 48 hours. The survival and apoptosis rates of those cells were estimated by MTT assay and fluorescein isothiocyanate (FITC)-annexin V/propidium Iodide (PI) flow cytometry respectively.

RESULTS

EPO induced a stable improvement of neurite outgrowth of retinal neurocytes in a dose-dependent manner. Compared with the control group, the neurite outgrowth length increased to 162.8% at 6.0 U/ml EPO exposure. EPO had no any significant effect on the survival and apoptosis rates of the retinal neurocytes cultured in serum-free media, but it was beneficial in promoting the survival and decreasing the early and total apoptosis rates of the cultured retinal neurocytes suffering from glutamate-induced cytotoxicity.

CONCLUSION

EPO had a significant biological effect on neurite outgrowth of the dissociated retinal neurocytes in vitro. EPO was beneficial in promoting the survival and decreasing the apoptosis rates of the cultured retinal neurocytes suffering from glutamate-induced cytotoxicity.

摘要

目的

阐明促红细胞生成素(EPO)对培养的视网膜神经细胞神经突生长的影响,并研究EPO是否可能对保护遭受谷氨酸诱导细胞毒性的培养视网膜神经细胞有益。

方法

视网膜神经细胞培养48小时后,将培养基换成无血清培养基,并将培养的视网膜细胞分别暴露于1.0 U/ml、3.0 U/ml和6.0 U/ml的EPO中再培养48小时;然后用苏丹黑B对细胞进行染色,并用图像分析系统评估这些细胞的神经突生长情况。视网膜神经细胞培养48小时后,将细胞培养于含有5 mM或10 mM谷氨酸的无血清培养基中,并分别在有或无Epo(1.0 U/ml、3.0 U/ml、6.0 U/ml)存在的情况下再培养48小时。分别通过MTT法和异硫氰酸荧光素(FITC)-膜联蛋白V/碘化丙啶(PI)流式细胞术评估这些细胞的存活率和凋亡率。

结果

EPO以剂量依赖性方式稳定促进视网膜神经细胞的神经突生长。与对照组相比,在6.0 U/ml EPO作用下神经突生长长度增加至162.8%。EPO对在无血清培养基中培养的视网膜神经细胞的存活率和凋亡率无显著影响,但对遭受谷氨酸诱导细胞毒性的培养视网膜神经细胞的存活有促进作用,并降低其早期和总凋亡率。

结论

EPO对体外分离的视网膜神经细胞的神经突生长有显著生物学作用。EPO对遭受谷氨酸诱导细胞毒性的培养视网膜神经细胞的存活有促进作用,并降低其凋亡率。

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