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Proteomic profiling of nuclei from native renal inner medullary collecting duct cells using LC-MS/MS

机译:使用LC-MS / MS从天然肾脏内髓收集管细胞中对细胞核进行蛋白质组学分析

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摘要

Vasopressin is a peptide hormone that regulates renal water excretion in part through its actions on the collecting duct. The regulation occurs in part via control of transcription of genes coding for the water channels aquaporin-2 (Aqp2) and aquaporin-3 (Aqp3). To identify transcription factors expressed in collecting duct cells, we have carried out LC-MS/MS-based proteomic profiling of nuclei isolated from native rat inner medullary collecting ducts (IMCDs). To maximize the number of proteins identified, we matched spectra to rat amino acid sequences using three different search algorithms (SEQUEST, InsPecT, and OMSSA). All searches were coupled to target-decoy methodology to limit false-discovery identifications to 2% of the total for single-peptide identifications. In addition, we developed a computational tool (ProMatch) to identify and eliminate ambiguous identifications. With this approach, we identified >3,500 proteins, including 154 proteins classified as “transcription factor” proteins (Panther Classification System). Among these, are members of CREB, ETS, RXR, NFAT, HOX, GATA, EBOX, EGR, MYT1, KLF, and CP2 families, which were found to have evolutionarily conserved putative binding sites in the 5′-flanking region or first intron of the Aqp2 gene, as well as members of EBOX, NR2, GRE, MAZ, KLF, and SP1 families corresponding to conserved sites in the 5′-flanking region of the Aqp3 gene. In addition, several novel phosphorylation sites in nuclear proteins were identified using the neutral loss-scanning LC-MS3 technique. The newly identified proteins have been incorporated into the IMCD Proteome Database ().
机译:加压素是一种肽激素,部分地通过其对收集管的作用来调节肾水的排泄。该调节部分通过控制编码水通道aquaporin-2(Aqp2)和aquaporin-3(Aqp3)的基因的转录而发生。为了鉴定在收集管细胞中表达的转录因子,我们对从天然大鼠内髓样收集管(IMCD)分离出的核进行了基于LC-MS / MS的蛋白质组分析。为了最大化鉴定出的蛋白质数量,我们使用三种不同的搜索算法(SEQUEST,InsPecT和OMSSA)将光谱与大鼠氨基酸序列进行匹配。所有搜索都与目标诱骗方法相结合,以将错误发现的识别数限制为单肽识别总数的2%。此外,我们开发了一种计算工具(ProMatch)来识别和消除模棱两可的标识。通过这种方法,我们鉴定出3500种以上的蛋白质,其中154种蛋白质被归类为“转录因子”蛋白质(Panther分类系统)。其中包括CREB,ETS,RXR,NFAT,HOX,GATA,EBOX,EGR,MYT1,KLF和CP2家族的成员,这些成员在5'侧翼区域或第一内含子中具有进化保守的推定结合位点。 Aqp2基因的“基因”以及EBOX,NR2,GRE,MAZ,KLF和SP1家族的成员,它们对应于Aqp3基因5'侧翼区域的保守位点。此外,使用中性损失扫描LC-MS 3 技术鉴定了核蛋白中的几个新的磷酸化位点。新鉴定的蛋白质已被整合到IMCD蛋白质组数据库()中。

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