Department of Anatomy, Institute of Biology, University of Campinas (UNICAMP), CP 6109, CEP 13083-970, Campinas, SP, Brazil.
J Neuroinflammation. 2010 May 24;7:31. doi: 10.1186/1742-2094-7-31.
Astrocytes play a major role in preserving and restoring structural and physiological integrity following injury to the nervous system. After peripheral axotomy, reactive gliosis propagates within adjacent spinal segments, influenced by the local synthesis of nitric oxide (NO). The present work investigated the importance of inducible nitric oxide synthase (iNOS) activity in acute and late glial responses after injury and in major histocompatibility complex class I (MHC I) expression and synaptic plasticity of inputs to lesioned alpha motoneurons.
In vivo analyses were carried out using C57BL/6J-iNOS knockout (iNOS(-/-)) and C57BL/6J mice. Glial response after axotomy, glial MHC I expression, and the effects of axotomy on synaptic contacts were measured using immunohistochemistry and transmission electron microscopy. For this purpose, 2-month-old animals were sacrificed and fixed one or two weeks after unilateral sciatic nerve transection, and spinal cord sections were incubated with antibodies against classical MHC I, GFAP (glial fibrillary acidic protein - an astroglial marker), Iba-1 (an ionized calcium binding adaptor protein and a microglial marker) or synaptophysin (a presynaptic terminal marker). Western blotting analysis of MHC I and nNOS expression one week after lesion were also performed. The data were analyzed using a two-tailed Student's t test for parametric data or a two-tailed Mann-Whitney U test for nonparametric data.
A statistical difference was shown with respect to astrogliosis between strains at the different time points studied. Also, MHC I expression by iNOS(-/-) microglial cells did not increase at one or two weeks after unilateral axotomy. There was a difference in synaptophysin expression reflecting synaptic elimination, in which iNOS(-/-) mice displayed a decreased number of the inputs to alpha motoneurons, in comparison to that of C57BL/6J.
The findings herein indicate that iNOS isoform activity influences MHC I expression by microglial cells one and two weeks after axotomy. This finding was associated with differences in astrogliosis, number of presynaptic terminals and synaptic covering of alpha motoneurons after lesioning in the mutant mice.
星形胶质细胞在神经系统损伤后维持和恢复结构和生理完整性方面发挥着重要作用。在外周轴突切断后,反应性神经胶质增生在相邻的脊髓节段内传播,受局部合成的一氧化氮(NO)的影响。本研究调查了诱导型一氧化氮合酶(iNOS)活性在损伤后急性和晚期神经胶质反应以及主要组织相容性复合体 I 类(MHC I)表达和损伤的α运动神经元传入突触可塑性中的重要性。
使用 C57BL/6J-iNOS 敲除(iNOS(-/-)) 和 C57BL/6J 小鼠进行体内分析。使用免疫组织化学和透射电子显微镜测量轴突切断后的神经胶质反应、神经胶质 MHC I 表达以及轴突切断对突触接触的影响。为此,在单侧坐骨神经横断后 1 或 2 周处死 2 个月大的动物,并使用针对经典 MHC I、GFAP(胶质纤维酸性蛋白-星形胶质细胞标志物)、Iba-1(离子钙结合衔接蛋白和小胶质细胞标志物)或突触小体蛋白(突触前末端标志物)的抗体孵育脊髓切片。还对损伤后 1 周 MHC I 和 nNOS 表达进行 Western 印迹分析。使用参数数据的双尾学生 t 检验或非参数数据的双尾曼-惠特尼 U 检验分析数据。
在不同研究时间点,不同菌株之间的星形胶质细胞增生存在统计学差异。另外,iNOS(-/-)小胶质细胞的 MHC I 表达在单侧轴突切断后 1 或 2 周时没有增加。突触小体蛋白表达存在差异,反映了突触消除,与 C57BL/6J 相比,iNOS(-/-)小鼠的α运动神经元输入数量减少。
本研究结果表明,iNOS 同工酶活性影响轴突切断后 1 至 2 周时小胶质细胞的 MHC I 表达。这一发现与突变小鼠损伤后神经胶质增生、突触前末端数量和α运动神经元突触覆盖的差异有关。
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