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기정민

Kee, Jung-Min
Bioorganic and Chembio Lab.
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dc.citation.conferencePlace KO -
dc.citation.conferencePlace 부산 벡스코 -
dc.citation.title 128회 대한화학회 학술발표회 -
dc.contributor.author Jung, Hoyoung -
dc.contributor.author Kee, Jung-Min -
dc.date.accessioned 2024-01-31T21:36:10Z -
dc.date.available 2024-01-31T21:36:10Z -
dc.date.created 2021-11-16 -
dc.date.issued 2021-10-14 -
dc.description.abstract Protein Arg phosphorylation is a crucial post-translational modification (PTM) for stress response, virulence, and protein quality control of Gram-positive bacteria. Although this PTM was first discovered in the 1970s, it is only recently that a protein Arg kinase (McsB) and a pArg phosphatase (YwlE) have been identified in Gram-positive bacteria. McsB marks misfolded protein by Arg phosphorylation, and the pArg tag is recognized by the bacterial proteasome for degradation, analogous to protein ubiquitination in eukaryotes. Recently, we reported a CHEF-based fluorescent probe for real-time monitoring of Arg kinase/phosphatase activities in vitro. However, the peptide-based probe was not applicable to live-cell studies. To overcome this limitation, we developed new genetically encoded FRET-based enzyme activity probes for studying Arg phosphorylation dynamics in live cells. This sensor should be invaluable in studying the regulatory mechanisms of Arg phosphorylation dynamics. -
dc.identifier.bibliographicCitation 128회 대한화학회 학술발표회 -
dc.identifier.uri https://scholarworks.unist.ac.kr/handle/201301/76926 -
dc.publisher 대한화학회 -
dc.title A genetically encoded fluorescent sensor for protein Arg phosphorylation dynamics in live cells -
dc.type Conference Paper -
dc.date.conferenceDate 2021-10-13 -

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