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  Delayed Times to Tissue Fixation Result in Unpredictable Global Phosphoproteome Changes

Guendisch, S., Grundner-Culemann, K., Wolff, C., Schott, C., Reischauer, B., Machatti, M., Groelz, D., Schaab, C., Tebbe, A., & Becker, K.-F. (2013). Delayed Times to Tissue Fixation Result in Unpredictable Global Phosphoproteome Changes. JOURNAL OF PROTEOME RESEARCH, 12(10), 4424-4434. doi:10.1021/pr400451z.

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資料種別: 学術論文

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 作成者:
Guendisch, Sibylle1, 著者
Grundner-Culemann, Kathrin1, 著者
Wolff, Claudia1, 著者
Schott, Christina1, 著者
Reischauer, Bilge1, 著者
Machatti, Manuela1, 著者
Groelz, Daniel1, 著者
Schaab, Christoph2, 著者           
Tebbe, Andreas1, 著者
Becker, Karl-Friedrich1, 著者
所属:
1external, ou_persistent22              
2Mann, Matthias / Proteomics and Signal Transduction, Max Planck Institute of Biochemistry, Max Planck Society, ou_1565159              

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キーワード: BREAST-CANCER PATIENTS; PROTEIN MICROARRAYS; SIGNALING NETWORKS; MASS-SPECTROMETRY; PHOSPHORYLATION; HER2; PROTEOMICS; STABILITY; PATHWAYS; SILACtissue; preanalytical phase; protein; biomarker; biobank; RPPA; phosphoproteomics; mass spectrometry;
 要旨: Protein phosphorylation controls the activity of signal transduction pathways regulated by kinases and phosphatases. Little is known, however, about the impact of preanalytical factors, for example, delayed times to tissue fixation, on global phosphoprotein levels in tissues. The aim of this study was to characterize the potential effects of delayed tissue preservation (cold ischemia) on the levels of phosphoproteins using targeted and nontargeted proteomic approaches. Rat and murine liver samples were exposed to different cold ischemic conditions ranging from 10 to 360 min prior to cryopreservation. The phosphoproteome was analyzed using reverse phase protein array (RPPA) technology and phosphoprotein-enriched quantitative tandem mass spectrometry (LC-MS/MS). RPPA analysis of rat liver tissues with long (up to 360 min) cold ischemia times did not reveal statistically significant alterations of specific phosphoproteins even though nonphosphorylated cytokeratin 18 (CK18) showed increased levels after 360 min of delay to freezing. Keeping the samples on ice prior to cryopreservation prevented this effect. LC-MS/MS-based quantification of 1684 phosphorylation sites in rat liver tissues showed broadening of their distribution compared to time point zero, but without reaching statistical significance for individual phosphosites. Similarly, RPPA analysis of mouse liver tissues with short (<60 min) cold ischemia times did not reveal directed or predictable changes of protein and phosphoprotein levels. Using LC-MS/MS and quantification of 791 phosphorylation sites, we found that the distribution of ratios compared to time point zero broadens with prolonged ischemia times, but these were rather undirected and diffuse changes, as we could not detect significant alterations of individual phosphosites. On the basis of our results from RPPA and LC-MS/MS analysis of rat and mouse liver tissues, we conclude that prolonged cold ischemia results in unspecific phosphoproteome changes that can be neither predicted nor assigned to individual proteins. On the other hand, we identified a number of phosphosites which were extraordinarily stable even after 360 min of cold ischemia and, therefore, may be used as general reference markers for future companion diagnostics for kinase inhibitors.

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言語: eng - English
 日付: 2013-10
 出版の状態: 出版
 ページ: 11
 出版情報: -
 目次: -
 査読: 査読あり
 識別子(DOI, ISBNなど): ISI: 000326320300014
DOI: 10.1021/pr400451z
 学位: -

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出版物名: JOURNAL OF PROTEOME RESEARCH
種別: 学術雑誌
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出版社, 出版地: 1155 16TH ST, NW, WASHINGTON, DC 20036 USA : AMER CHEMICAL SOC
ページ: - 巻号: 12 (10) 通巻号: - 開始・終了ページ: 4424 - 4434 識別子(ISBN, ISSN, DOIなど): ISSN: 1535-3893