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dc.contributor.author Bae, Jingi ko
dc.contributor.author Kim, Su-Jin ko
dc.contributor.author Lee, Seung-Eun ko
dc.contributor.author Kwon, Wooil ko
dc.contributor.author Kim, Hongbeom ko
dc.contributor.author Han, Youngmin ko
dc.contributor.author Jang, Jin-Young ko
dc.contributor.author Kim, Min-Sik ko
dc.contributor.author Lee, Sang-Won ko
dc.date.accessioned 2019-05-09T06:55:37Z -
dc.date.available 2019-05-09T06:55:37Z -
dc.date.created 2019-05-09 -
dc.date.issued 2019-04 -
dc.identifier.citation Clinical Proteomics, v.16, no.1 -
dc.identifier.issn 1542-6416 -
dc.identifier.uri http://hdl.handle.net/20.500.11750/9829 -
dc.description.abstract Certain tumors such as pancreatic ductal adenocarcinoma (PDAC) are known to contain a variety of hydrolytic enzymes including RNases and proteases that may lead to degradation of RNA and proteins during sample processing. For such tumor tissues with RNA instability, RNAlater containing a high concentration of quaternary ammonium sulfates that denature RNA-hydrolyzing enzymes is often used to protect RNAs from hydrolysis. Although a few studies have been carried out to determine the effect of RNAlater on DNA and RNA, whether RNAlater influences the proteome and phosphoproteome is largely unknown. In this study we carried out a systematic and comprehensive analysis of the effect of RNAlater on the proteome and phosphoproteome using high-resolution mass spectrometry. PDAC tissues from three patients were individually pulverized and the tissue powders of each patient were divided into two portions, one of which was incubated in RNAlater at 4 °C for 24 h (RNAlater tissue) while the other was kept at - 80 °C (frozen tissue). Comprehensive quantitative profiling experiments on the RNAlater tissues and the frozen tissues resulted in the identification of 99,136 distinct peptides of 8803 protein groups and 17,345 phosphopeptides of 16,436 phosphosites. The data exhibited no significant quantitative changes in both proteins and phosphorylation between the RNAlater tissues and the frozen tissue. In addition, the phosphoproteome data showed heterogeneously activated pathways among the three patients that were not altered by RNAlater. These results indicate that the tissue preservation method using RNAlater can be effectively used on PDAC tissues for proteogenomic studies where preservation of intact DNA, RNA and proteins is prerequisite. Data from this study are available via ProteomeXchange with the identifier PXD010710. © 2019 The Author(s). -
dc.language English -
dc.publisher BMC -
dc.title Comprehensive proteome and phosphoproteome profiling shows negligible influence of RNAlater on protein abundance and phosphorylation -
dc.type Article -
dc.identifier.doi 10.1186/s12014-019-9239-z -
dc.identifier.wosid 000465935400001 -
dc.identifier.scopusid 2-s2.0-85065251086 -
dc.type.local Article(Overseas) -
dc.type.rims ART -
dc.description.journalClass 1 -
dc.contributor.nonIdAuthor Bae, Jingi -
dc.contributor.nonIdAuthor Kim, Su-Jin -
dc.contributor.nonIdAuthor Lee, Seung-Eun -
dc.contributor.nonIdAuthor Kwon, Wooil -
dc.contributor.nonIdAuthor Kim, Hongbeom -
dc.contributor.nonIdAuthor Han, Youngmin -
dc.contributor.nonIdAuthor Jang, Jin-Young -
dc.contributor.nonIdAuthor Lee, Sang-Won -
dc.identifier.citationVolume 16 -
dc.identifier.citationNumber 1 -
dc.identifier.citationTitle Clinical Proteomics -
dc.type.journalArticle Article -
dc.description.isOpenAccess Y -
dc.subject.keywordPlus PROTEOGENOMIC CHARACTERIZATION -
dc.subject.keywordPlus COMPUTATIONAL PLATFORM -
dc.subject.keywordPlus SNAP-FROZEN -
dc.subject.keywordPlus HUMAN COLON -
dc.subject.keywordPlus RNA -
dc.subject.keywordPlus DNA -
dc.contributor.affiliatedAuthor Kim, Min-Sik -
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Department of New Biology Laboratory for QBIO and Precision Medicine 1. Journal Articles

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