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Chae, Young Chan
Cancer Translational Research Lab.
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dc.citation.endPage 1266 -
dc.citation.number 9 -
dc.citation.startPage 1257 -
dc.citation.title TRANSPLANTATION -
dc.citation.volume 86 -
dc.contributor.author Lee, Sukmook -
dc.contributor.author Ha, In Su -
dc.contributor.author Kim, Jae Hyeon -
dc.contributor.author Park, Kyong Soo -
dc.contributor.author Han, Kyu Hyun -
dc.contributor.author Kim, Sun-Hee -
dc.contributor.author Chae, Young Chan -
dc.contributor.author Kim, Sun Hee -
dc.contributor.author Kim, Yun Hee -
dc.contributor.author Suh, Pann-Ghill -
dc.contributor.author Ryu, Sung Ho -
dc.contributor.author Kim, Jung-Eun -
dc.contributor.author Bang, Kitae -
dc.contributor.author Hwang, Jong-Ik -
dc.contributor.author Yang, Jaeseok -
dc.contributor.author Park, Kwang-Wook -
dc.contributor.author Chung, Junho -
dc.contributor.author Ahn, Curie -
dc.date.accessioned 2023-12-22T08:16:00Z -
dc.date.available 2023-12-22T08:16:00Z -
dc.date.created 2015-01-12 -
dc.date.issued 2008-11 -
dc.description.abstract Background. The use of porcine islets as alternatives to transplantable human islets is hampered by xenotransplant rejection. To identify molecular mechanisms that would allow subversion of xenoislet rejection, we investigated the role of H2O2 in vascular cell adhesion molecule-1 (VCAM-1) expression by porcine and mouse islets and beta-cell lines.
Methods. Porcine islets were treated with H2O2, tumor necrosis factor alpha, interferon-gamma, interleukin-1 beta, and lipopolysaccharide, to assess the effects of inflammatory stimulators on VCAM-1 expression using flow cytometry. The role of Ca2+ in H2O2-induced VCAM-1 expression was investigated in beta-cell lines using an extracellular Ca2+ chelator and Ca2+-depleted media. Furthermore, H2O2-induced VCAM-1 expression was measured in beta-cells, pretreated with inhibitors of protein kinase C, phospholipase D, and phosphatidylinositol-3 kinase/Akt. Finally, H2O2-induced VCAM-1 expression was evaluated in porcine islets and rodent beta-cell lines infected with an adenovirus encoding catalase, a H2O2-removing enzyme.
Results. H2O2 was most potent inflammatory stimulator of VCAM-1 expression in porcine islets and had the greatest effect on VCAM-1 expression by beta-cells. Signaling pathway analysis demonstrated that extracellular Ca2+ influx was critical to H2O2-mediated VCAM-1 expression; however, protein kinase C, phospholipase D, and phosphatidylinositol-3 kinase/Akt activation were not required for VCAM-1 expression. Finally, catalase overexpression inhibited H2O2-induced VCAM-1 expression by islets and beta-cell lines.
Conclusion. An extracellular calcium-dependent H2O2 pathway is the critical mediator of VCAM-1 expression by pancreatic islets and beta-cells. Inhibition of this pathway by catalase overexpression in donor islets can be exploited to protect against xenoislet immune responses.
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dc.identifier.bibliographicCitation TRANSPLANTATION, v.86, no.9, pp.1257 - 1266 -
dc.identifier.doi 10.1097/TP.0b013e318188ab04 -
dc.identifier.issn 0041-1337 -
dc.identifier.scopusid 2-s2.0-58149149955 -
dc.identifier.uri https://scholarworks.unist.ac.kr/handle/201301/10096 -
dc.identifier.url http://www.scopus.com/inward/record.url?partnerID=HzOxMe3b&scp=58149149955 -
dc.identifier.wosid 000260945600016 -
dc.language 영어 -
dc.publisher LIPPINCOTT WILLIAMS & WILKINS -
dc.title Hydrogen Peroxide-Induced VCAM-1 Expression in Pancreatic Islets and beta-Cells Through Extracellular Ca2+ Influx -
dc.type Article -
dc.description.journalRegisteredClass scopus -
dc.subject.keywordAuthor Hydrogen peroxide -
dc.subject.keywordAuthor VCAM-1 -
dc.subject.keywordAuthor Pancreatic beta-cells -
dc.subject.keywordAuthor Calcium -
dc.subject.keywordAuthor Catalase -
dc.subject.keywordPlus NF-KAPPA-B -
dc.subject.keywordPlus NONSELECTIVE CATION CHANNEL -
dc.subject.keywordPlus SMOOTH-MUSCLE-CELLS -
dc.subject.keywordPlus OXIDATIVE
STRESS
-
dc.subject.keywordPlus ALLOGRAFT-REJECTION -
dc.subject.keywordPlus ENDOTHELIAL-CELLS -
dc.subject.keywordPlus ADHESION MOLECULE-1 -
dc.subject.keywordPlus NADPH OXIDASE -
dc.subject.keywordPlus GLUTATHIONE-PEROXIDASE -
dc.subject.keywordPlus SUPEROXIDE-DISMUTASE -

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