运动通过改善PD模型小鼠纹状体D2MSN-D1MSN侧抑制效应调节基底神经节信息输出

赵刚; 刘晓莉; 乔德才

doi:10.16469/j.css.202001006

运动通过改善PD模型小鼠纹状体D2MSN-D1MSN侧抑制效应调节基底神经节信息输出

Exercise Improves the Lateral Inhibition of D2MSN-D1MSN in the Striatum to Regulate Basal Ganglia Information Output in Parkinson’s Disease Mice

摘要

摘要: 目的:通过研究运动及多巴胺Ⅱ型受体(dopamine type Ⅱ receptor,D2R)激动剂干预对PD模型小鼠纹状体D2MSN-D1MSN侧抑制效应的影响,揭示运动在改善PD小鼠基底神经节信息输出中的作用及机制。方法:选用4周龄雄性D2-Cre小鼠,右侧纹状体注射兴奋性光敏感蛋白病毒(rAAV-Ef1α-DIO-ChR2-EYFP-WPRE-pA),通过光遗传技术精准操控D2MSN。小鼠随机分为对照组(D2-Cre)和模型组,纹状体分别注射生理盐水和神经毒素6-羟基多巴胺(6-Hydroxydopamine hydrobromide,6-OHDA),经鉴定符合PD标准的模型组小鼠再分为PD组(PD^D2-Cre)和PD运动组(PD+Ex^D2-Cre)。采用4周匀速跑台运动(18 m/min,40 min/天,连续5天/周)和D2R激动剂分别对各组小鼠进行干预。实验结束后,制备离体脑片,利用全细胞膜片钳结合光遗传技术检测各组小鼠纹状体D2MSN-D1MSN侧抑制效应及黑质网状部的信息输出,并验证侧抑制效应的变化是否由D2R介导。结果:光刺激D2-MSN后,D1-MSN动作电位发放个数PD^D2-Cre组显著低于D2-Cre组(P<0.05);PD+Ex^D2-Cre组显著高于PD^D2-Cre组,但仍低于D2-Cre组(P<0.05)。光刺激D2-MSN诱发D1-MSN抑制性突触后电流(Optogenetic stimulation evoked inhibitory postsynaptic currents,oIPSC)的幅值与基线比值,PD^D2-Cre组显著高于D2-Cre组(P<0.05),PD+Ex^D2-Cre组显著低于PD^D2-Cre组,但高于D2-Cre组(P<0.05);光刺激D2-MSN诱发黑质网状部(SNr)抑制性突触后场电位(field inhibitory post synaptic potential,fIPSP)最大幅值,PD^D2-Cre组显著低于D2-Cre组(P<0.05),PD+Ex^D2-Cre组显著高于PD^D2-Cre组,但低于D2-Cre组(P<0.05)。结论:PD模型小鼠纹状体D2MSN-D1MSN侧抑制效应异常,并影响了SNr的信息输出,这可能是导致PD基底神经节功能紊乱的重要原因之一。4周运动干预通过改善PD模型小鼠纹状体D2MSN-D1MSN侧抑制效应,调节了SNr的信息输出。D2R在运动改善PD小鼠纹状体D2MSN-D1MSN侧抑制效应和调节基底神经节信息输出中起重要作用。

Abstract: Objective: To investigate the role and mechanism of striatum D2MSN-D1MSN lateral inhibition in improving basal ganglia information output by observing the effects of exercise and dopamine type Ⅱ receptor(D2R) agonist intervention on the inhibition of striatum D2MSN-D1MSN in PD mice. Methods: D2-Cre mice were microinjected with Optogenetic viral(rAAV-Ef1α-DIO-ChR2-EYFP-WPRE-pA) into right striatum to optogenetic manipulate D2MSN, then the mice were randomly divided into a control group(D2-Cre) and a model group. The PD mice model was established by injecting neurotoxin 6-OHDA into the striatum with 6-Hydroxydopamine hydrobromide(6-OHDA) in two weeks, while the control group was injected saline at the same position.The PD mice were identified and then randomly divided into PD group(PD^D2-Cre) and PD exercise group(PD+Ex^D2-Cre). The constant speed treadmill exercise(18 m/min, 40 min/d, 5 d/w) for 4 weeks or D2R agonist was set as intervention method in each group. After intervention, striatum D2MSN-D1MSN lateral inhibition was examined by whole cell patch clamp combined with optogenetic technique. The D2R agonist was applied to examine whether the lateral inhibition change depends on D2R or not. Results: The number of D1-MSNs action potentials in the PD^D2-Cre group was significantly lower than the D2-Cre group(P<0.05); the PD+Ex^D2-Cre group was significantly higher than that of PD+Ex^D2-Cregroup and lower than D2-Cre group(P<0.05). Using D2R agonist drug characteristics to interfere with D2-MSNs, the ratio of oIPSC amplitude to baseline in D1-MSNs of PD^D2-Cregroup was significantly higher than the D2-Cre group(P<0.05), and PD+Ex^D2-Cregroup was significantly lower than PD^D2-Cregroup, but higher than the D2-Cre group(P<0.05); the maximal field inhibitory post synaptic potential(fIPSP)amplitude of SNr induced by optogeneticstimulate D2-MSN in PD^D2-Cregroup was significantly lower than the D2-Cre group(P<0.05). PD+Ex^D2-Cregroup was significantly higher than PD^D2-Cre group, but lower than the D2-Cre group(P<0.05). Conclusion: The abnormal lateral inhibition affects the information output of SNr in PD mice, which may be one of the important mechanism of PD basal ganglia dysfunction. Four-week exercise intervention adjusted the SNr information output by improving the D2MSN-D1MSN lateral inhibition in the striatum of PD mice,and D2R plays an important role in exercise-improved D2MSN-D1MSN lateral inhibition and the regulation of basal ganglia information output.

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