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Exogenous modulation of intrinsic optic nerve neuroprotective activity.

机译:内在视神经神经保护活性的外源调节。

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BACKGROUND: To characterize the molecular and functional status of the rat retina and optic nerve after acute elevation of intraocular pressure (IOP). METHODS: Retinal ischemia was induced in rats by increasing the IOP (110 mmHg/60 minutes). Microarray analysis, quantitative RT-PCR (qRT-PCR) and immunohistochemistry were used to characterize retinal tissue. PLGA microspheres containing neurotrophic factors (BDNF, GDNF, or CNTF) or empty microspheres were injected into the vitreous of operated animals 1 day after elevation of IOP. Pupil light reflex (PLR) parameters and electroretinograms (ERG) were monitored at multiple time points during the 60-day postoperative recovery period. RESULTS: Molecular analysis showed a significant intrinsic up-regulation of CNTF at 10 and 25 days after induction of the acute ocular hypertension (p = 0.0067). Molecular tissue analysis of GDNF and its receptors (GDNFR1, GDNFR2), and BDNF and its receptor (trkB) showed no change in expression. Animals that received CNTF microspheres had no significant functional recovery compared to animals which received blank microspheres (p > 0.05). Animals that received GDNF or BDNF microspheres showed significant PLR recovery (p < 0.05 and p < 0.001 respectively) compared to non-treated animals. CONCLUSIONS: Continuous release of neurotrophic growth factors (NGFs) significantly protects optic nerve function in the experimental model of retinal ischemia observed by PLR analysis.
机译:背景:表征急性眼内压升高后大鼠视网膜和视神经的分子和功能状态。方法:通过增加眼压(110 mmHg / 60分钟)来诱导大鼠视网膜缺血。微阵列分析,定量RT-PCR(qRT-PCR)和免疫组织化学被用来表征视网膜组织。在IOP升高1天后,将含有神经营养因子(BDNF,GDNF或CNTF)的PLGA微球或空微球注入手术动物的玻璃体中。在术后60天恢复期的多个时间点,监测瞳孔的光反射(PLR)参数和视网膜电图(ERG)。结果:分子分析显示,在诱发急性高眼压后10天和25天,CNTF的内在显着上调(p = 0.0067)。 GDNF及其受体(GDNFR1,GDNFR2)和BDNF及其受体(trkB)的分子组织分析显示表达没有变化。与接受空白微球的动物相比,接受CNTF微球的动物没有明显的功能恢复(p> 0.05)。与未治疗的动物相比,接受GDNF或BDNF微球的动物表现出显着的PLR恢复(分别为p <0.05和p <0.001)。结论:通过PLR分析观察,在视网膜缺血实验模型中,神经营养生长因子(NGFs)的持续释放显着保护视神经功能。

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