Regulation of mitochondrial motility and mitophagy by LRRK2.

LRRK2 对线粒体运动和线粒体自噬的调节。

• 批准号: 8800524
• 负责人: XINNAN WANG
• 金额: $ 39.85万
• 依托单位: STANFORD UNIVERSITY
• 依托单位国家: 美国
• 财政年份: 2014
• 资助国家: 美国
• 起止时间: 2014-09-30 至 2019-07-31
• 项目状态: 已结题
• 来源: https://reporter.nih.gov/project-details/8800524
• 关键词: Affect; Axon; Binding; Biochemical; Biology; Cell physiology; Cell-Free System; Cells; Complex; Cultured Cells; Defect; Drosophila genus; Economics; Equilibrium; Fibroblasts; Genes; Genetic; Inherited; Kinesin; LRRK2 gene; Laboratories; Length; Link; Mediating; Microtubules; Mission; Mitochondria; Mitochondrial Membrane Protein; Modeling; Molecular; Motor; Movement; Mutation; Neurobiology; Neurodegenerative Disorders; Neurons; Outer Mitochondrial Membrane; Oxidative Stress; PINK1 gene; PTEN-induced putative kinase; Parkinson Disease; Pathogenesis; Pathway interactions; Patients; Phenotype; Phosphotransferases; Pluripotent Stem Cells; Protein Binding; Proteins; Public Health; Recruitment Activity; Regulation; Research Proposals; Rodent Model; Testing; Therapeutic Intervention; United States National Institutes of Health; cell motility; effective therapy; in vivo; insight; mutant; nervous system disorder; novel; parkin gene/protein; polarized cell; post-doctoral training; prevent; protein degradation; public health relevance

DESCRIPTION (provided by applicant): Anterograde mitochondrial transport in neuronal axons is mediated by a primary motor/adaptor complex which includes motor protein KHC (kinesin heavy chain), and two mitochondrial adaptors milton and Miro (Glater et al., 2006). In the current model, Miro, an outer mitochondrial membrane (OMM) protein, binds to milton which in turn binds to KHC, to recruit mitochondria to motors and microtubules (Guo et al., 2005, Fransson et al., 2006, Glater et al., 2006). During my postdoctoral training, I discovered that two PD proteins PINK1 and Parkin target Miro for degradation to promote damage-induced mitophagy (Wang et al., 2011). This is consistent with our preliminary observation conducted in my own laboratory that mutant Parkin fibroblasts from one PD patient are failed to degrade Miro after mitochondrial damage and are impaired in mitophagy. The most common genetic form of hereditary PD is caused by a G2019S mutation in the LRRK2 gene. LRRK2 encodes a multi-domain Ser/Thr kinase with unknown functions and unconfirmed substrates. Surprisingly, we found that Miro is also retained on damaged mitochondria in fibroblasts from one PD patient with LRRK2G2019S. In addition, we have preliminary evidence that in LRRK2G2019S iPSC (inducible pluripotent stem cells)-derived neurons from two PD patients, damaged mitochondria fail to stop and to undergo mitophagy, reminiscent of those found in mutant PINK1 or Parkin rodent models (Wang et al., 2011). Therefore, LRRK2G2019S, just like PINK1 or Parkin mutations, prevents Miro protein from degradation on damaged mitochondria, disrupting mitochondrial motility and mitophagy. However, there has been no evidence directly linking LRRK2 to Miro and mitochondrial transport. What is the mechanism underlying the same phenotype caused by distinct PD mutations? In this proposal, we aim to unravel this puzzle. We hypothesize that LRRK2 and PINK1/Parkin operate in parallel pathways but eventually converge on the common substrate Miro. In an alternative model, LRRK2 may not directly phosphorylate Miro, but rather it could genetically or physically interact with and regulate PINK1 or Parkin to control damaged mitochondrial transport and clearance by influencing turn-over of Miro. The molecular mechanism we will define in this research proposal will provide insight into LRRK2-related PD pathogenesis, especially for patients with LRRK2G2019S, which represents about 5-6% of the total cases (Bonifati, 2006). In addition to its relevance to PD, we also expect our results elucidating the mechanisms underlying neuronal mitochondrial transport and clearance to illuminate basic principles of mitochondrial biology and neurobiology. Thus, we propose to use a combination of Drosophila genetics, cultured cells, and even PD patient fibroblasts and derived neurons to pursue the following Specific Aims. Aim 1: To determine the mechanism by which LRRK2 influences the turnover of Miro. Aim 2: To determine the physical relationship between LRRK2 and Miro. Aim 3: To dissect the relationship between LRRK2 and the PINK1/Parkin pathway.

描述（由申请人提供）：神经元轴突的顺行线粒体运输由初级运动/接头复合物介导，该复合物包括运动蛋白KHC（运动蛋白重链）和两个线粒体接头milton和Miro （Glater et al., 2006）。在目前的模型中，线粒体外膜（OMM）蛋白Miro与milton结合，而milton又与KHC结合，将线粒体招募到马达和微管中（Guo等人，2005年，Fransson等人，2006年，Glater等人，2006年）。在我的博士后训练中，我发现了两个