CPEB1 directs muscle stem cell activation by reprogramming the translational landscape

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作者
Wenshu Zeng
Lu Yue
Kim S. W. Lam
Wenxin Zhang
Wai-Kin So
Erin H. Y. Tse
Tom H. Cheung
机构
[1] The Hong Kong University of Science and Technology,Division of Life Science
[2] The Hong Kong University of Science and Technology,Center for Stem Cell Research
[3] The Hong Kong University of Science and Technology,HKUST
[4] The Hong Kong University of Science and Technology,Nan Fung Life Science Joint Laboratory
[5] The Hong Kong University of Science and Technology,State Key Laboratory of Molecular Neuroscience
[6] Hong Kong Center for Neurodegenerative Diseases,Molecular Neuroscience Center
[7] Disease and Drug Development,Guangdong Provincial Key Laboratory of Brain Science
[8] Shenzhen-Hong Kong Institute of Brain Science,undefined
[9] HKUST Shenzhen Research Institute,undefined
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Skeletal muscle stem cells, also called Satellite Cells (SCs), are actively maintained in quiescence but can activate quickly upon extrinsic stimuli. However, the mechanisms of how quiescent SCs (QSCs) activate swiftly remain elusive. Here, using a whole mouse perfusion fixation approach to obtain bona fide QSCs, we identify massive proteomic changes during the quiescence-to-activation transition in pathways such as chromatin maintenance, metabolism, transcription, and translation. Discordant correlation of transcriptomic and proteomic changes reveals potential translational regulation upon SC activation. Importantly, we show Cytoplasmic Polyadenylation Element Binding protein 1 (CPEB1), post-transcriptionally affects protein translation during SC activation by binding to the 3′ UTRs of different transcripts. We demonstrate phosphorylation-dependent CPEB1 promoted Myod1 protein synthesis by binding to the cytoplasmic polyadenylation elements (CPEs) within its 3′ UTRs to regulate SC activation and muscle regeneration. Our study characterizes CPEB1 as a key regulator to reprogram the translational landscape directing SC activation and subsequent proliferation.
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