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dc.contributor.author하정미-
dc.date.accessioned2019-05-20T04:28:31Z-
dc.date.available2019-05-20T04:28:31Z-
dc.date.issued2008-07-
dc.identifier.citationJOURNAL OF THE AMERICAN CHEMICAL SOCIETY, v. 130, No. 32, Page. 10474-10475en_US
dc.identifier.issn0002-7863-
dc.identifier.urihttps://pubs.acs.org/doi/abs/10.1021/ja803395d-
dc.identifier.urihttps://repository.hanyang.ac.kr/handle/20.500.11754/104717-
dc.description.abstractLight-activatable ("caged") proteins have been used to correlate, with exquisite temporal and spatial control, intracellular biochemical action with global cellular behavior. However, the chemical or genetic construction of caged proteins is nontrivial, with subsequent laborious introduction into living cells, potentially problematic competition with natural endogenous counterparts, and challenging intracellular incorporation at levels equivalent to the natural enzymes. We describe the design, synthesis, and characterization of small molecular equivalents of a caged Src kinase. These compounds are easy to prepare and function by inhibiting the action of the natural unmodified enzyme.en_US
dc.language.isoen_USen_US
dc.publisherAMER CHEMICAL SOCen_US
dc.subjectCATALYTIC SUBUNITen_US
dc.subjectTYROSINE KINASESen_US
dc.subjectACQUISITIONen_US
dc.titleLight-Mediated Liberation of Enzymatic Activity: "Small Molecule" Caged Protein Equivalentsen_US
dc.typeArticleen_US
dc.relation.volume130-
dc.identifier.doi10.1021/ja803395d-
dc.relation.page10474-10475-
dc.relation.journalJOURNAL OF THE AMERICAN CHEMICAL SOCIETY-
dc.contributor.googleauthorLi, Haishan-
dc.contributor.googleauthorHah, Jung-Mi-
dc.contributor.googleauthorLawrence, David S.-
dc.relation.code2008205895-
dc.sector.campusE-
dc.sector.daehakCOLLEGE OF PHARMACY[E]-
dc.sector.departmentDEPARTMENT OF PHARMACY-
dc.identifier.pidjhah-
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COLLEGE OF PHARMACY[E](약학대학) > PHARMACY(약학과) > Articles
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