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整合转录组和蛋白质组分析揭示了人类脑类器官中核糖体基因的转录后调控。

Integrated transcriptome and proteome analysis reveals posttranscriptional regulation of ribosomal genes in human brain organoids.

机构信息

Institute of Molecular Biotechnology of the Austrian Academy of Sciences (IMBA), Vienna BioCenter (VBC), Vienna, Austria.

Gregor Mendel Institute, Vienna Biocenter, Vienna, Austria.

出版信息

Elife. 2023 Mar 29;12:e85135. doi: 10.7554/eLife.85135.

Abstract

During development of the human cerebral cortex, multipotent neural progenitors generate excitatory neurons and glial cells. Investigations of the transcriptome and epigenome have revealed important gene regulatory networks underlying this crucial developmental event. However, the posttranscriptional control of gene expression and protein abundance during human corticogenesis remains poorly understood. We addressed this issue by using human telencephalic brain organoids grown using a dual reporter cell line to isolate neural progenitors and neurons and performed cell class and developmental stage-specific transcriptome and proteome analysis. Integrating the two datasets revealed modules of gene expression during human corticogenesis. Investigation of one such module uncovered mTOR-mediated regulation of translation of the 5'TOP element-enriched translation machinery in early progenitor cells. We show that in early progenitors partial inhibition of the translation of ribosomal genes prevents precocious translation of differentiation markers. Overall, our multiomics approach proposes novel posttranscriptional regulatory mechanisms crucial for the fidelity of cortical development.

摘要

在人类大脑皮层发育过程中,多能神经祖细胞产生兴奋性神经元和神经胶质细胞。对转录组和表观基因组的研究揭示了这一关键发育事件背后重要的基因调控网络。然而,人类皮质发生过程中基因表达和蛋白质丰度的转录后调控仍知之甚少。我们使用双报告细胞系培养的人类端脑类器官来解决这个问题,以分离神经祖细胞和神经元,并进行细胞类和发育阶段特异性转录组和蛋白质组分析。整合这两个数据集揭示了人类皮质发生过程中的基因表达模块。对其中一个模块的研究揭示了 mTOR 介导的早期祖细胞中富含 5'TOP 元件的翻译机器翻译的调节。我们表明,在早期祖细胞中,核糖体基因翻译的部分抑制可防止分化标志物的过早翻译。总的来说,我们的多组学方法提出了新的转录后调控机制,对皮质发育的保真度至关重要。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/be8b/10059687/4ccdabf599f3/elife-85135-fig1.jpg

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