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首页> 外文期刊>Nucleic Acids Research >Genome-wide single-cell-level screen for protein abundance and localization changes in response to DNA damage in S-cerevisiae
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Genome-wide single-cell-level screen for protein abundance and localization changes in response to DNA damage in S-cerevisiae

机译:全基因组单细胞水平筛查蛋白含量和定位变化以响应S-酿酒酵母中的DNA损伤

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An effective response to DNA damaging agents involves modulating numerous facets of cellular homeostasis in addition to DNA repair and cell-cycle checkpoint pathways. Fluorescence microscopy-based imaging offers the opportunity to simultaneously interrogate changes in both protein level and subcellular localization in response to DNA damaging agents at the single-cell level. We report here results from screening the yeast Green Fluorescent Protein (GFP)-fusion library to investigate global cellular protein reorganization on exposure to the alkylating agent methyl methanesulfonate (MMS). Broad groups of induced, repressed, nucleus- and cytoplasm-enriched proteins were identified. Gene Ontology and interactome analyses revealed the underlying cellular processes. Transcription factor (TF) analysis identified principal regulators of the response, and targets of all major stress-responsive TFs were enriched amongst the induced proteins. An unexpected partitioning of biological function according to the number of TFs targeting individual genes was revealed. Finally, differential modulation of ribosomal proteins depending on methyl methanesulfonate dose was shown to correlate with cell growth and with the translocation of the Sfp1 TF. We conclude that cellular responses can navigate different routes according to the extent of damage, relying on both expression and localization changes of specific proteins.
机译:对DNA破坏剂的有效反应除了调节DNA修复和细胞周期检查点途径外,还涉及调节细胞稳态的许多方面。基于荧光显微镜的成像提供了同时询问蛋白质水平和亚细胞定位变化的机会,以响应单细胞水平的DNA损伤剂。我们在这里报告筛选酵母绿色荧光蛋白(GFP)融合文库的结果,以调查暴露于烷基化剂甲磺酸甲酯(MMS)时的全球细胞蛋白重组。鉴定了广泛的诱导,抑制,细胞核和细胞质富集蛋白。基因本体论和相互作用组分析揭示了潜在的细胞过程。转录因子(TF)分析确定了反应的主要调控因子,并且所有主要的应激反应TF的靶标都富含诱导蛋白。根据针对单个基因的TF的数量,发现了生物学功能的意外分配。最后,依赖于甲磺酸甲酯的剂量,核糖体蛋白的差异调节显示与细胞生长和Sfp1 TF的易位相关。我们得出结论,细胞反应可以根据损伤的程度来导航不同的路径,这取决于特定蛋白质的表达和定位变化。

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