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活海马神经元中轴突 β-肌动蛋白 mRNA 的动力学。

Dynamics of axonal β-actin mRNA in live hippocampal neurons.

机构信息

Department of Physics and Astronomy, Seoul National University, Seoul, Republic of Korea.

Department of Mechanical Engineering, Seoul National University, Seoul, Republic of Korea.

出版信息

Traffic. 2022 Oct;23(10):496-505. doi: 10.1111/tra.12865. Epub 2022 Aug 31.

Abstract

Localization of mRNA facilitates spatiotemporally controlled protein expression in neurons. In axons, mRNA transport followed by local protein synthesis plays a critical role in axonal growth and guidance. However, it is not yet clearly understood how mRNA is transported to axonal subcellular sites and what regulates axonal mRNA localization. Using a transgenic mouse model in which endogenous β-actin mRNA is fluorescently labeled, we investigated β-actin mRNA movement in axons of hippocampal neurons. We cultured neurons in microfluidic devices to separate axons from dendrites and performed single-particle tracking of axonal β-actin mRNA. Compared with dendritic β-actin mRNA, axonal β-actin mRNA showed less directed motion and exhibited mostly subdiffusive motion, especially near filopodia and boutons in mature dissociated hippocampal neurons. We found that axonal β-actin mRNA was likely to colocalize with actin patches (APs), regions that have a high density of filamentous actin (F-actin) and are known to have a role in branch initiation. Moreover, simultaneous imaging of F-actin and axonal β-actin mRNA in live neurons revealed that moving β-actin mRNA tended to be docked in the APs. Our findings reveal that axonal β-actin mRNA localization is facilitated by actin networks and suggest that localized β-actin mRNA plays a potential role in axon branch formation.

摘要

mRNA 的定位有助于神经元中时空控制的蛋白质表达。在轴突中,mRNA 的运输随后进行局部蛋白质合成,在轴突生长和导向中起着关键作用。然而,目前尚不清楚 mRNA 如何被运输到轴突亚细胞部位,以及什么调节轴突 mRNA 的定位。利用内源性β-肌动蛋白 mRNA 荧光标记的转基因小鼠模型,我们研究了海马神经元轴突中β-肌动蛋白 mRNA 的运动。我们将神经元在微流控装置中培养,将轴突与树突分离,并对轴突β-肌动蛋白 mRNA 进行单颗粒追踪。与树突β-肌动蛋白 mRNA 相比,轴突β-肌动蛋白 mRNA 的定向运动较少,表现出更多的亚扩散运动,特别是在成熟分离的海马神经元的丝状伪足和末梢中。我们发现,轴突β-肌动蛋白 mRNA 可能与肌动蛋白斑(APs)共定位,APs 是丝状肌动蛋白(F-actin)密度较高的区域,已知在分支起始中起作用。此外,在活神经元中同时对 F-actin 和轴突β-肌动蛋白 mRNA 进行成像显示,移动的β-肌动蛋白 mRNA 倾向于停靠在 APs 中。我们的发现表明,轴突β-肌动蛋白 mRNA 的定位是由肌动蛋白网络促进的,并表明局部化的β-肌动蛋白 mRNA 在轴突分支形成中可能发挥作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ef03/9804286/e13e28376518/TRA-23-496-g003.jpg

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