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dc.contributor.authorKim, YJ-
dc.contributor.authorCha, SS-
dc.contributor.authorKim, JS-
dc.contributor.authorShin, NK-
dc.contributor.authorJeong, WJ-
dc.contributor.authorShin, HC-
dc.contributor.authorOh, BH-
dc.contributor.authorHahn, JH-
dc.date.accessioned2016-03-31T13:44:24Z-
dc.date.available2016-03-31T13:44:24Z-
dc.date.created2009-02-28-
dc.date.issued1999-02-15-
dc.identifier.issn0003-2697-
dc.identifier.other1999-OAK-0000000615-
dc.identifier.urihttps://oasis.postech.ac.kr/handle/2014.oak/20496-
dc.description.abstractElectrospray ionization mass spectrometry (ESI-MS) is employed to directly analyze the limited trypsinolysis products of wild-type tumor necrosis factor-alpha (wtTNF-alpha) and its mutant, M3S. To determine the charge numbers of peaks of relatively small peptides in the ESI mass spectrum of a digest, a series of sodium-adduct ion peaks of each peptide are generated by adding a small quantity of NaCl to the digest before taking the spectrum. From the monitoring of the composition of proteolytic mixture as the incubation time is lengthened, it has been learned that the proteolysis of wtTNF-alpha by trypsin occurs sequentially: Arg(2), Arg(6), Arg(32), Arg(31), and Arg(44), and that M3S is strongly resistant to the proteolysis. Since the cleavage sequence of wtTNF-alpha and the mutation-induced resistance of M3S are consistent with the structural features of the proteins, we can suggest a mutant more resistant to proteolysis than M3S, which has an additional point mutation, Ala35Leu or Ala35Ile. (C) 1999 Academic Press.-
dc.description.statementofresponsibilityX-
dc.languageEnglish-
dc.publisherACADEMIC PRESS INC-
dc.relation.isPartOfANALYTICAL BIOCHEMISTRY-
dc.subjectSTRUCTURAL CHARACTERIZATION-
dc.subjectBINDING PROTEIN-
dc.subjectPROTEOLYSIS-
dc.subjectIDENTIFICATION-
dc.subjectSITE-
dc.titleDetermination of the limited trypsinolysis pathways of tumor necrosis factor-alpha and its mutant by electrospray ionization mass spectrometry-
dc.typeArticle-
dc.contributor.college화학과-
dc.identifier.doi10.1006/abio.1998.2999-
dc.author.googleKIM, YJ-
dc.author.googleCHA, SS-
dc.author.googleKIM, JS-
dc.author.googleSHIN, NK-
dc.author.googleJEONG, WJ-
dc.author.googleSHIN, HC-
dc.author.googleOH, BH-
dc.author.googleHAHN, JH-
dc.relation.volume267-
dc.relation.issue2-
dc.relation.startpage279-
dc.relation.lastpage286-
dc.contributor.id10082554-
dc.relation.journalANALYTICAL BIOCHEMISTRY-
dc.relation.indexSCI급, SCOPUS 등재논문-
dc.relation.sciSCI-
dc.collections.nameJournal Papers-
dc.type.rimsART-
dc.identifier.bibliographicCitationANALYTICAL BIOCHEMISTRY, v.267, no.2, pp.279 - 286-
dc.identifier.wosid000078674600005-
dc.date.tcdate2019-01-01-
dc.citation.endPage286-
dc.citation.number2-
dc.citation.startPage279-
dc.citation.titleANALYTICAL BIOCHEMISTRY-
dc.citation.volume267-
dc.contributor.affiliatedAuthorOh, BH-
dc.contributor.affiliatedAuthorHahn, JH-
dc.identifier.scopusid2-s2.0-0345390294-
dc.description.journalClass1-
dc.description.journalClass1-
dc.description.wostc1-
dc.type.docTypeArticle-
dc.subject.keywordPlusIDENTIFICATION-
dc.subject.keywordPlusSITE-
dc.subject.keywordPlusSTRUCTURAL CHARACTERIZATION-
dc.subject.keywordPlusBINDING PROTEIN-
dc.subject.keywordPlusPROTEOLYSIS-
dc.relation.journalWebOfScienceCategoryBiochemical Research Methods-
dc.relation.journalWebOfScienceCategoryBiochemistry & Molecular Biology-
dc.relation.journalWebOfScienceCategoryChemistry, Analytical-
dc.description.journalRegisteredClassscie-
dc.description.journalRegisteredClassscopus-
dc.relation.journalResearchAreaBiochemistry & Molecular Biology-
dc.relation.journalResearchAreaChemistry-

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오병하OH, BYUNG HA
Dept of Life Sciences
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