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A Systematic RNAi Screen Reveals a Novel Role of a Spindle Assembly Checkpoint Protein BuGZ in Synaptic Transmission in C. elegans

机译:系统的RNAi屏幕揭示线轴装配检查点蛋白BuGZ在秀丽隐杆线虫的突触传递中的新型作用。

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摘要

Synaptic vesicles (SV) store various neurotransmitters that are released at the synapse. The molecular mechanisms of biogenesis, exocytosis, and endocytosis for SV, however, remain largely elusive. In this study, using Complex Object Parametric Analysis and Sorter (COPAS) to monitor the fluorescence of synapto-pHluorin (SpH), we performed a whole-genome RNAi screen in C. elegans to identify novel genetic modulators in SV cycling. One hundred seventy six genes that up-regulating SpH fluorescence and 96 genes that down-regulating SpH fluorescence were identified after multi-round screen. Among these genes, B0035.1 (bugz-1) encodes ortholog of mammalian C2H2 zinc-finger protein BuGZ/ZNF207, which is a spindle assembly checkpoint protein essential for mitosis in human cells. Combining electrophysiology, imaging and behavioral assays, we reveal that depletion of BuGZ-1 results in defects in locomotion. We further demonstrate that BuGZ-1 promotes SV recycling by regulating the expression levels of endocytosis-related genes such as rab11.1. Therefore, we have identified a bunch of potential genetic modulators in SV cycling, and revealed an unexpected role of BuGZ-1 in regulating synaptic transmission.
机译:突触小泡(SV)存储在突触处释放的各种神经递质。然而,SV的生物发生,胞吐作用和胞吞作用的分子机制仍然很难捉摸。在这项研究中,使用复杂对象参数分析和分类器(COPAS)来监测突触pHluorin(SpH)的荧光,我们在秀丽隐杆线虫中进行了全基因组RNAi筛选,以鉴定SV循环中的新型遗传调节剂。经过多轮筛选,鉴定出176个上调SpH荧光的基因和96个下调SpH荧光的基因。在这些基因中,B0035.1(bugz-1)编码哺乳动物C2H2锌指蛋白BuGZ / ZNF207的直系同源物,这是人类细胞有丝分裂必不可少的纺锤体组装检查点蛋白。结合电生理学,成像和行为分析,我们揭示BuGZ-1耗竭导致运动缺陷。我们进一步证明,BuGZ-1通过调节内吞相关基因如rab11.1的表达水平来促进SV回收。因此,我们在SV循环中发现了一堆潜在的基因调节剂,并揭示了BuGZ-1在调节突触传递中的意外作用。

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