Induction of GD3/α1-adrenergic receptor/transglutaminase 2-mediated erythroid differentiation in chronic myelogenous leukemic K562 cells

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dc.contributor.authorS H Ha-
dc.contributor.authorS K Kang-
dc.contributor.authorH Choi-
dc.contributor.authorC H Kwak-
dc.contributor.authorF Abekura-
dc.contributor.authorJ Y Park-
dc.contributor.authorK M Kwon-
dc.contributor.authorH W Chang-
dc.contributor.authorY C Lee-
dc.contributor.authorK T Ha-
dc.contributor.authorBo Kyeng Hou-
dc.contributor.authorT W Chung-
dc.contributor.authorC H Kim-
dc.date.accessioned2018-01-11-
dc.date.available2018-01-11-
dc.date.issued2017-
dc.identifier.issn1949-2553-
dc.identifier.urihttps://oak.kribb.re.kr/handle/201005/17471-
dc.description.abstractThe disialic acid-containing glycosphingolipid GD3 recruited membrane transglutaminase 2 (TG2) as a signaling molecule for erythroid differentiation in human chronic myelogenous leukemia (CML) K562 cells. The α1-adrenergic receptor (α1-AR)/TG2-mediated signaling pathway regulated GD3 functions, including gene expression and production, to differentiate CML K562 cells into erythroid lineage cells. Epinephrine, an AR agonist, increased membrane recruitment as well as GTP-photoaffinity of TG2, inducing GD3 synthase gene expression. Epinephrine activated PI3K/Akt signaling and GTPase downstream of TG2 activated Akt. The coupling of TG2 and GD3 production was specifically suppressed by prazosin (α1-AR antagonist), but not by propranolol (β-AR antagonist) or rauwolscine (α2-AR antagonist), indicating α1-AR specificity. Small interfering RNA (siRNA) experiment results indicated that the α1-AR/TG2-mediated signaling pathway activated PKCs α and δ to induce GD3 synthase gene expression. Transcription factors CREB, AP-1, and NF-κB regulated GD3 synthase gene expression during α1-AR-induced differentiation in CML K562 cells. In addition, GD3 synthase gene expression was upregulated in TG2-transfected cells via α1-AR with expression of erythroid lineage markers and benzidine-positive staining. α1-AR/TG2 signaling pathway-directed GD3 production is a crucial step in erythroid differentiation of K562 cells and GD3 interacts with α1-AR/TG2, inducing GD3/α1-AR/TG2-mediated erythroid differentiation. These results suggest that GD3, which acts as a membrane mediator of erythroid differentiation in CML cells, provides a therapeutic avenue for leukemia treatment.-
dc.publisherImpact Journalsko
dc.titleInduction of GD3/α1-adrenergic receptor/transglutaminase 2-mediated erythroid differentiation in chronic myelogenous leukemic K562 cells-
dc.title.alternativeInduction of GD3/α1-adrenergic receptor/transglutaminase 2-mediated erythroid differentiation in chronic myelogenous leukemic K562 cells-
dc.typeArticle-
dc.citation.titleOncotarget-
dc.citation.number42-
dc.citation.endPage72219-
dc.citation.startPage72205-
dc.citation.volume8-
dc.contributor.affiliatedAuthorBo Kyeng Hou-
dc.contributor.alternativeName하선형-
dc.contributor.alternativeName강성구-
dc.contributor.alternativeName최현주-
dc.contributor.alternativeName곽충환-
dc.contributor.alternativeNameAbekura-
dc.contributor.alternativeName박준영-
dc.contributor.alternativeName권경민-
dc.contributor.alternativeName장현욱-
dc.contributor.alternativeName이영춘-
dc.contributor.alternativeName하기태-
dc.contributor.alternativeName허보경-
dc.contributor.alternativeName정태욱-
dc.contributor.alternativeName김철호-
dc.identifier.bibliographicCitationOncotarget, vol. 8, no. 42, pp. 72205-72219-
dc.identifier.doi10.18632/oncotarget.20080-
dc.subject.keywordadrenergic receptor-
dc.subject.keyworderythroid differentiation-
dc.subject.keywordganglioside GD3-
dc.subject.keywordhuman chronic myelogenous leukemia K562 cell-
dc.subject.keywordtransglutaminase 2-
dc.subject.localadrenergic receptor-
dc.subject.localErythroid differentiation-
dc.subject.localerythroid differentiation-
dc.subject.localGanglioside GD3-
dc.subject.localganglioside GD3-
dc.subject.localhuman chronic myelogenous leukemia K562 cell-
dc.subject.localtransglutaminase 2-
dc.subject.localTransglutaminase 2-
dc.subject.localTransglutaminase II-
dc.description.journalClassN-
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