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在全营养、无血清饥饿和雷帕霉素处理条件下,人源神经元型一氧化氮合酶/一氧化氮合酶1(nNOS/NOS1)阳性与对照SH-SY5Y神经母细胞瘤细胞的深度蛋白质组。

Deep proteome of human nNOS/NOS1-positive versus MOCK SH-SY5Y neuroblastoma cells under full nutrition, serum free starvation and rapamycin treatment.

作者信息

Heidler Juliana, Valek Lucie, Wittig Ilka, Tegeder Irmgard

机构信息

Functional Proteomics, SFB815 Core Unit, Goethe-University, Frankfurt, Germany.

Institute of Clinical Pharmacology, Goethe-University Hospital, Frankfurt, Germany.

出版信息

Data Brief. 2018 Oct 26;21:1309-1314. doi: 10.1016/j.dib.2018.10.079. eCollection 2018 Dec.

Abstract

Upregulations of neuronal nitric oxide synthase (nNOS/NOS1) in the mouse brain upon aging suggest a role in age-associated changes of protein homeostasis. We generated a cell model, in which constitutive expression of nNOS in SH-SY5Y cells at a level comparable to mouse brain replicates the aging phenotype i.e. slowing of cell proliferation, cell enlargement and expression of senescence markers. nNOS+ and MOCK cells were exposed to proteostasis stress by treatment with rapamycin or serum-free starvation. The proteomes were analyzed per SILAC or label-free using hybrid liquid chromatography/mass spectrometry (LC/MS). Full scan MS-data were acquired using Xcalibur, and raw mass spectra were analyzed using the proteomics software MaxQuant. The human reference proteome from uniprot was used as template to identify peptides and proteins and quantify protein expression. The DiB data file contains essential MaxQuant output tables and includes peptide and protein identification, accession numbers, protein and gene names, sequence coverage and quantification values of each sample. Differences in protein expression in MOCK versus nNOS+ SH-SY5Y cells and interpretation of results are presented in Valek et al. (2018). Raw mass spectra and MaxQuant output files have been deposited to the ProteomeXchange Consortium (Vizcaino et al., 2014) via the PRIDE partner repository with the dataset identifier PRIDE: PXD010538.

摘要

衰老过程中小鼠大脑中神经元型一氧化氮合酶(nNOS/NOS1)的上调表明其在蛋白质稳态的年龄相关变化中发挥作用。我们构建了一个细胞模型,其中SH-SY5Y细胞中nNOS的组成性表达水平与小鼠大脑相当,复制了衰老表型,即细胞增殖减慢、细胞增大和衰老标志物的表达。通过用雷帕霉素处理或无血清饥饿使nNOS+和MOCK细胞暴露于蛋白质稳态应激。使用混合液相色谱/质谱(LC/MS)通过SILAC或无标记分析蛋白质组。使用Xcalibur采集全扫描MS数据,并使用蛋白质组学软件MaxQuant分析原始质谱。来自uniprot的人类参考蛋白质组用作鉴定肽和蛋白质以及量化蛋白质表达的模板。DiB数据文件包含重要的MaxQuant输出表,包括肽和蛋白质鉴定、登录号、蛋白质和基因名称、每个样品的序列覆盖率和量化值。MOCK与nNOS+ SH-SY5Y细胞中蛋白质表达的差异以及结果解释见Valek等人(2018年)。原始质谱和MaxQuant输出文件已通过PRIDE合作伙伴存储库存入蛋白质组交换联盟(Vizcaino等人,2014年),数据集标识符为PRIDE:PXD010538。

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