川芎提取物通过miR-23a-3p/SNCA轴对帕金森综合征模型MPP^(+)诱导的SH-SY5Y细胞的影响

目的探究川芎提取物对MPP^(+)诱导的SH-SY5Y细胞和帕金森综合征的影响。方法1-甲基-4苯基吡啶离子(MPP^(+))干预SH-SY5Y建立帕金森综合征细胞模型(SH-SY5Y-MPP^(+)),川芎提取物干预后检测细胞增殖、凋亡以及miR-23a-3p、SNCA的表达情况。另观察调控miR-23a-3p、SNCA表达后SH-SY5Y-MPP^(+)的变化,双荧光素报告酶验证miR-23a-3p与SNCA的关系。结果SH-SY5Y-MPP^(+)的细胞增殖能力明显低于SH-SY5Y,而凋亡率则高于SH-SY5Y(P<0.05)。川芎提取物干预下,SH-SY5Y-MPP^(+)的增殖能力、Bcl-2、SNCA蛋白升高,凋亡率与miR-23a-3p、Bax蛋白降低(P<0.05)。沉默miR-23a-3p与升高SNCA均可以促进SH-SY5Y-MPP^(+)的增殖能力,抑制凋亡;而升高miR-23a-3p与沉默SNCA则反之(P<0.05)。在线靶基因预测网站发现,miR-23a-3p与SNCA存在可结合的互补位点,双荧光素报告酶显示SNCA-wt的萤火活性在转染了miR-23a-3p模拟物序列后受到了明显的抑制(P<0.05)。在升高miR-23a-3p后,SH-SY5Y-MPP^(+)中SNCA蛋白表达降低,而沉默miR-23a-3p则反之(P<0.05)。拯救实验显示,川芎提取物对SH-SY5Y-MPP^(+)的干预效果被升高miR-23a-3p或沉默SNCA完全逆转(P>0.05);升高miR-23a-3p对SH-SY5Y-MPP^(+)产生的影响则升高SNCA逆转(P>0.05)。结论川芎提取物通过调控miR-23a-3p/SNCA轴影响MPP^(+)诱导的SH-SY5Y生物学行为改变,未来可能是治疗帕金森综合征的新方向。

五味子酚对MPP^＋诱导的SH-SY5Y细胞凋亡的保护作用

帕金森病（Parkinson’s disease，PD）目前发病率较高，尚无理想的治疗药物。从抗氧化剂中寻找神经保护剂已成为防治PD的新途径，是目前国际上研究的热点。五味子酚（schisanhenol，Sal）是五味子的有效成分，具有显著的抗氧化活性和神经细胞保护作用。

MPP^+诱导SK-N-SH细胞热休克蛋白的表达研究

目的研究SK-N-SH细胞在受到1-甲基-4-苯基-吡啶离子(MPP+)损伤时,细胞内热休克蛋白(HSPs)的表达。方法SK-N-SH细胞中加入不同浓度的MPP+制备帕金森病(PD)细胞模型,分别于培养24 h和48 h时,检测细胞存活率,选择合适的MPP+实验浓度。免疫印迹法(W estern b lot)和免疫细胞化学法观察细胞内Hsp70、Hsp40(HD J-1和HD J-2)和Hsp90的变化。结果细胞存活率检测表明MPP+合适的实验浓度为10~500μmol/L。W estern b lot和免疫细胞化学法检测均显示250μmol/L MPP+处理24 h,细胞内Hsp70含量明显升高(P<0.05);MPP+处理48 h,Hsp70含量随MPP+浓度的升高而下降;Hsp40/HD J-1和Hsp90的变化趋势基本与Hsp70相同;而HD J-2在细胞内的含量无明显改变(P>0.05)。结论HSPs的含量在MPP+制备的PD细胞模型中,随MPP+作用时间的延长而呈现先增加后降低的趋势。

Effect of total isoflavones from pueraria lobata on the expressions of preproenkephalin, prodynorphin and D2 dopamine receptor mRNA in PC12 cells induced by MPP^+

Objective： The aim of the study was to observe the effect of total isoflavones from pueraria Iobata （TIP） on D2 dopamine receptor mRNA, preproenkephalin mRNA and prodynorphin mRNA expressions in Parkinson＇s disease （PD） model cells induced by 1-methyl-4-phenylpyridinium ion （MPP^＋）. Methods： TIP was dissolved in 0.1 M NaOH and added to the culture medium at a final concentrations of 50 mg/L, 100 mg/L and 200 mg/L. Some cells （control） were exposed to 0.001 M NaOH. TIP was added to PC12 cells 30 min prior to the administration of MPP^＋. TIP and MPP^＋ remained in the culture medium for 96 h. D2 dopamine receptor mRNA, preproenkephalin mRNA and prodynorphin mRNA expressions were assayed by real-time quantitative reverse transcription-PCR. Results： The D2 dopamine receptor mRNA and preproenkephalin mRNA expressions were up-regulated in MPP^＋ group compared with the control group, and prodynorphin mRNA expression was down-regulated in that. The D2 dopamine receptor mRNA expression being down-regulated and prodynorphin mRNA expression being up-regulated in TIP group compared with the MPP^＋ group. And there was no effect of TIP on preproenkephalin gene expression in PC12 cells induced by MPP^＋. Conclusion： The results suggest that TIP down-regulates the D2 dopamine receptor mRNA expression, up-regulates prodynorphin mRNA expression and not affects preproenkephalin gene expression in PC12 cells induced by MPP^＋.