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PNAS Plus: Optically triggering spatiotemporally confined GPCR activity in a cell and programming neurite initiation and extension

机译:PNAS Plus:以光学方式触发细胞中时空受限的GPCR活性并编程神经突的起始和延伸

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摘要

G-protein–coupled receptor (GPCR) activity gradients evoke important cell behavior but there is a dearth of methods to induce such asymmetric signaling in a cell. Here we achieved reversible, rapidly switchable patterns of spatiotemporally restricted GPCR activity in a single cell. We recruited properties of nonrhodopsin opsins—rapid deactivation, distinct spectral tuning, and resistance to bleaching—to activate native Gi, Gq, or Gs signaling in selected regions of a cell. Optical inputs were designed to spatiotemporally control levels of second messengers, IP3, phosphatidylinositol (3,4,5)-triphosphate, and cAMP in a cell. Spectrally selective imaging was accomplished to simultaneously monitor optically evoked molecular and cellular response dynamics. We show that localized optical activation of an opsin-based trigger can induce neurite initiation, phosphatidylinositol (3,4,5)-triphosphate increase, and actin remodeling. Serial optical inputs to neurite tips can refashion early neuron differentiation. Methods here can be widely applied to program GPCR-mediated cell behaviors.
机译:G蛋白偶联受体(GPCR)活性梯度引起重要的细胞行为,但缺乏诱导细胞中这种不对称信号转导的方法。在这里,我们在单个细胞中实现了时空限制的GPCR活性的可逆,快速切换模式。我们募集了非视紫红质视蛋白的特性-快速失活,独特的光谱调谐和对漂白的抵抗力-以激活细胞选定区域中的天然Gi,Gq或Gs信号传导。光学输入旨在时空控制细胞中第二信使,IP3,磷脂酰肌醇(3,4,5)-三磷酸和cAMP的水平。完成光谱选择性成像以同时监测光学诱发的分子和细胞反应动力学。我们显示基于视蛋白的触发器的局部光学激活可以诱导神经突起始,磷脂酰肌醇(3,4,5)-三磷酸酯增加和肌动蛋白重塑。神经突尖端的串行光学输入可以重新塑造早期的神经元分化。这里的方法可以广泛应用于编程GPCR介导的细胞行为。

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