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Joo, Jinmyoung
Laboratory for Advanced Biomaterials and Translational Medicine
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dc.citation.startPage 102242 -
dc.citation.title Nano Today -
dc.citation.volume 56 -
dc.contributor.author Pack, Chan-Gi -
dc.contributor.author Jung, Min Kyo -
dc.contributor.author Kim, Kyunghwan -
dc.contributor.author Yoo, Woojung -
dc.contributor.author Kim, Minjong -
dc.contributor.author Cho, Minju -
dc.contributor.author Kang, Myoung-Hee -
dc.contributor.author Lee, Sanghwa -
dc.contributor.author Im, Jisu -
dc.contributor.author Kim, In Ki -
dc.contributor.author Lee, Sang-Wook -
dc.contributor.author Kim, Jun Ki -
dc.contributor.author Joo, Jinmyoung -
dc.date.accessioned 2024-06-14T09:35:09Z -
dc.date.available 2024-06-14T09:35:09Z -
dc.date.created 2024-06-14 -
dc.date.issued 2024-06 -
dc.description.abstract Uptake and intracellular trafficking of nanoparticles are tightly regulated by their interactions with cellular organelles and physiological microenvironment. Although the dynamic physicochemical reactions at the interface of nanoparticles and cells ultimately determine the intracellular distribution and fate, microscopic tracing and quantitative analysis of the nanoparticles have been hampered by the limited resolution associated with individual nanoparticle trafficking. Herein, we report spatiotemporal investigations on autophagic clearance of biodegradable iron oxide-silica core-shell nanoparticles in terms of intracellular trafficking and ionic dissolution at a single cell level using multimodal imaging systems. By combining transmission electron microscopy and super-resolution confocal laser scanning microscopy with fluorescence correlation spectroscopy, the complementary imaging analysis exclusively shows the intracellular uptake, endosomal fusion and biodegradative clearance, leading to identify the step-by-step endocytic transport pathway and autophagic degradation pathways. Tracing the intracellular trafficking of nanoparticles reveals that they are spontaneously transported from endosomes to lysosomes, and transiently stimulate autophagy while maintaining cell viability. While protecting iron oxide core, the silica shell is gradually degraded during endocytosis and autophagic clearance, resulting in ionic dissolution of iron oxide in acidic environment. Moreover, burst reduction of ferric ions by adding ascorbic acid readily triggers acute ferroptosis owing to rapid supplement of ferrous ions and Fenton reaction in cancer cells. The complementary imaging strategy provides insights into the design of biocompatible nanomedicines for cellular delivery and the degradative mechanisms beyond the intracellular fate. -
dc.identifier.bibliographicCitation Nano Today, v.56, pp.102242 -
dc.identifier.doi 10.1016/j.nantod.2024.102242 -
dc.identifier.issn 1748-0132 -
dc.identifier.scopusid 2-s2.0-85189446386 -
dc.identifier.uri https://scholarworks.unist.ac.kr/handle/201301/82990 -
dc.language 영어 -
dc.publisher Elsevier BV -
dc.title Spatiotemporal tracking of intracellular nanoparticles using complementary imaging systems reveals acute ferroptosis triggered by burst reduction of ferric ions -
dc.type Article -
dc.description.isOpenAccess TRUE -
dc.type.docType Article -
dc.description.journalRegisteredClass scie -
dc.description.journalRegisteredClass scopus -
dc.subject.keywordAuthor Biodegradation -
dc.subject.keywordAuthor Bioimaging -
dc.subject.keywordAuthor Cellular uptake -
dc.subject.keywordAuthor Drug delivery systems -
dc.subject.keywordAuthor Ferroptosis -
dc.subject.keywordAuthor Nanomedicine -

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