A small-molecule activator of ULK1 that induces cytoprotective autophagy for Parkinson disease treatment

OBJECTIVE To discover a small-molecule activator of ULK1 for Parkinson disease treatment and exploreits potential mechanisms.METHODS Candidate ULK1 activator was found by using structure-based design and high-through put screening,then modified by chemical synthesis and screened by kinase and autophgic activities.The amino acid residues that key to the activation site of the best candidate ULK1 activator(BL-918) were determined by site-directed mutagenesis,as well as in vitro kinase assay,ADP-Glo kinase assay and surface plasmon resonance(SPR) analysis.The mechanisms of BL-918 induced cytoprotective autophagy were investigated by electron microscopy,fluorescence microscopy,Western blotting,co-immunoprecipitation assay,si RNA and GFP-LC3 plasmid transfections.The therapeutic effect of BL-918 was determined by MPTP-mouse model,including behavioral tests,the levels of dopamine and its derivatives,as well as immunofluorescence and Western blotting.The toxicity of BL-918 was assessed by blood sample analysis and hematoxylin-eosin staining.RESULTS We discovered a small molecule(BL-918) as a potent activator of ULK1 by structure-based drug design.Subsequently,some key amino acid residues(Arg18,Lys50,Asn86 and Tyr89) were found to be crucial to the binding pocket between ULK1 and BL-918,by site-directed mutagenesis.Moreover,we found that BL-918 could induce autophagy via the ULK complex in neuroblastoma SH-SY5Y cells.Intriguingly,this activator displayed a cytoprotective effect on MPP+-treated SH-SY5Y cells,as well as protected against MPTP-induced motor dysfunction and loss of dopaminergic neurons by targeting ULK1-modulated autophagy in mouse models of PD.CONCLUSION We discovered a novel ULK1 activator(BL-918) that potently activated ULK1.This activator could induce cytoprotective autophagy via the ULK1 complex in SH-SY5Y cells,and also exerted its neuroprotective effects by targeting ULK1-modulated autophagy in a MPTP-induced PD mouse model,which may serve as a candidate drug for future PD therapy.

力竭运动对小鼠骨骼肌细胞自噬的影响及相关调节机制研究

目的:研究力竭运动对C57BL/6小鼠骨骼肌细胞自噬的影响,并探讨AMPK在骨骼肌自噬中的作用和调节机制。方法:8周龄C57BL/6小鼠96只,随机分为AICAR注射组,力竭运动组,Compound C注射+力竭运动组及相应对照组。各组小鼠分别在AICAR注射后1h,2h和6h或在进行终强度为11m/min的力竭跑台运动后即刻,3h,6h,12h,24h取材,每组6只。通过ELISA法测定AMPK酶活性,采用Western Blot法测定p-ULK1,ATG 7,LC3,Beclin1和p62蛋白表达,免疫共沉淀法测定AMPK/ULK1结合量。结果:AICAR注射后1h时AMPK酶活性、p-ULK1、AMPK/ULK1结合量、LC3-I和LC3-II显著升高(P<0.05),LC3-II/LC3-I比值显著增大(P<0.01),ATG 7、Beclin1显著下降(P<0.05),p62变化不明显,2h时除LC3-II显著下降外(P<0.01),其余指标基本恢复;力竭运动组AMPK酶活性,p-ULK1、AMPK/ULK1结合量,LC3-I和LC3-II运动结束即刻增加非常显著(P<0.01),LC3-II/LC3-I比值显著增大(P<0.01),恢复期(3h、6h、12h、24h)显著下降(P<0.01),ATG 7、Beclin1和p62运动后即刻显著下降(P<0.05),恢复期ATG 7始终低于对照组,Beclin1和p62逐渐恢复;Compound C注射+力竭运动组AMPK活性,p-ULK1含量和AMPK/ULK1结合量基本不变,LC3-I,LC3-II和LC3-II/LC3-I比值在运动后变化同力竭组一致,但显著低于力竭组(P<0.05),ATG 7,Beclin1变化同力竭组,但显著高于力竭组(P<0.05),p62在运动后即刻显著升高,恢复期(3h、6h、12h、24h)显著下降(P<0.05)。结论:AMPK是骨骼肌内细胞自噬的重要调节因子,力竭运动可以通过AMPK/ULK1途径显著提高骨骼肌细胞自噬水平,但AMPK/ULK1并非是调节骨骼肌细胞自噬的唯一途径。

脾气虚证大鼠股四头肌线粒体自噬水平及AMPK/ULK1途径变化的研究

目的观察脾气虚证大鼠股四头肌线粒体自噬水平及腺苷酸活化蛋白激酶(AMPK)/UNC-51-类似自噬激活激酶1(ULK1)途径的变化,从线粒体方面研究"脾气虚四肢不用"的机制。方法运用饮食失节+劳倦法复制脾气虚证大鼠模型,随机分为对照组和脾气虚模型组(模型组),造模成功后取股四头肌,比色法检测三磷酸腺苷(ATP)含量;JC-1法检测线粒体膜电位(MMP);免疫荧光及印迹法(Western blot)法检测微管相关蛋白1轻链3-B (LC3 B)、选择性自噬接头蛋白(p62)表达水平及与线粒体共定位的量;Western blot法检测AMPKα及ULK1蛋白表达。结果与对照组比较,模型组股四头肌ATP、MMP下降(P<0.05,P<0.01);LC3B-II蛋白表达及与线粒体共定位增加(均P<0.01)、p62蛋白表达及与线粒体共定位减少(均P<0.01);p-AMPKα/AMPKα及p-ULK1/ULK1比值升高(均P<0.01)。结论 "脾气虚四肢不用"可能与AMPK/ULK1途径激活所致的线粒体自噬水平提高不足有关。