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在脊椎动物大脑中进行大规模的细胞类型特异性蛋白质合成成像。

Large-scale cell-type-specific imaging of protein synthesis in a vertebrate brain.

机构信息

Max Planck Institute for Brain Research, Frankfurt, Germany.

出版信息

Elife. 2020 Feb 24;9:e50564. doi: 10.7554/eLife.50564.

Abstract

Despite advances in methods to detect protein synthesis, it has not been possible to measure endogenous protein synthesis levels in vivo in an entire vertebrate brain. We developed a transgenic zebrafish line that allows for cell-type-specific labeling and imaging of nascent proteins in the entire animal. By replacing leucine with glycine in the zebrafish MetRS-binding pocket (MetRS-L270G), we enabled the cell-type-specific incorporation of the azide-bearing non-canonical-amino-acid azidonorleucine (ANL) during protein synthesis. Newly synthesized proteins were then labeled via 'click chemistry'. Using a Gal4-UAS-ELAV3 line to express MetRS-L270G in neurons, we measured protein synthesis intensities across the entire nervous system. We visualized endogenous protein synthesis and demonstrated that seizure-induced neural activity results in enhanced translation levels in neurons. This method allows for robust analysis of endogenous protein synthesis in a cell-type-specific manner, in vivo at single-cell resolution.

摘要

尽管在检测蛋白质合成的方法上已经取得了进展,但仍不可能在整个脊椎动物大脑中测量内源性蛋白质合成水平。我们开发了一种转基因斑马鱼系,可实现整个动物中新生蛋白的细胞类型特异性标记和成像。通过将亮氨酸替换为 MetRS 结合口袋中的甘氨酸(MetRS-L270G),我们能够在蛋白质合成过程中特异性地掺入带有叠氮基团的非典型氨基酸叠氮甲硫氨酸(ANL)。然后,通过“点击化学”对新合成的蛋白质进行标记。使用 Gal4-UAS-ELAV3 系在神经元中表达 MetRS-L270G,我们测量了整个神经系统中的蛋白质合成强度。我们可视化了内源性蛋白质合成,并证明癫痫发作引起的神经活动导致神经元中的翻译水平增强。该方法允许以细胞类型特异性的方式,在单细胞分辨率下,对体内的内源性蛋白质合成进行稳健的分析。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1376/7048392/0f414c92df9d/elife-50564-fig1.jpg

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