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dc.contributor.author Lee, Eun Hye -
dc.contributor.author Lee, Jun Nyung -
dc.contributor.author Park, Song -
dc.contributor.author Chun, So Young -
dc.contributor.author Yoon, Bo Hyun -
dc.contributor.author Chung, Jae-Wook -
dc.contributor.author Choi, Seock Hwan -
dc.contributor.author Kim, Bum Soo -
dc.contributor.author Kim, Hyun Tae -
dc.contributor.author Kim, Tae Hwan -
dc.contributor.author Yoo, Eun Sang -
dc.contributor.author Lee, Sangkyu -
dc.contributor.author Choi, Jae Young -
dc.contributor.author Kwon, Tae Gyun -
dc.contributor.author Ha, Yun-Sok -
dc.date.accessioned 2022-11-15T12:10:11Z -
dc.date.available 2022-11-15T12:10:11Z -
dc.date.created 2022-07-22 -
dc.date.issued 2022-07 -
dc.identifier.issn 1875-6867 -
dc.identifier.uri http://hdl.handle.net/20.500.11750/17127 -
dc.description.abstract Background: Prostate cancer is the second most common cause of cancer related death in males worldwide. Most patients show no response to androgen deprivation therapy in case of recurrence and proceed to advanced stage with metastasis. TRPM7 is reported to be upregulated in diverse types of tumors. Methods: We analyzed the expression of TRPM7 and related proteins by Western blotting analysis. We performed cell migration and invasion assay to analyze the relationship between tumor aggressiveness and TRPM7. In addition, we proceeded an animal study by using stable TRPM7 knockdown cell line in xenograft. Results: In our results, TRPM7 regulates prostate cancer cell biology including proliferation, migration and invasion through ERK1/2, PI3K/Akt and JNK signaling pathways. We produced stable TRPM7 knockdown prostate cancer cell line. To analyze the relationship between TRPM7 and tumorigenesis, we proceeded migration and invasion assay as well as xenograft model. TRPM7 down-regulated DU145 cells showed suppressed migratory and invasion ability, 0.65- and 0.05-fold, respectively. In addition, we confirmed that the anti-cancer effect of TRPM7 is mediated through inactivation of ERK1/2, Src and Akt signaling pathways by western blotting analysis. P-ERK1/2, p-Src, and p-Akt expressions were reduced to 0.66-, 0.68-, and 0.66-fold, respectively. Moreover, we treated ERK, Akt and Src inhibitors to clarify the involvement of related each protein in migration and invasion ability, and we could observe that inhibitor treated cells showed suppressed migration and invasion ability. In vivo, TRPM7 knockdown cells projected decreased cell proliferation rate. Conclusions: Taken these results together, out study suggested TRPM7 might be an essential gene for prostate cancer metastasis by regulating prostate cancer cell proliferation, migration and invasion ability. -
dc.language English -
dc.publisher Elsevier BV -
dc.title Inhibition of TRPM7 suppresses migration and invasion of prostate cancer cells via inactivation of ERK1/2, Src and Akt pathway signaling -
dc.type Article -
dc.identifier.doi 10.31083/j.jomh1807144 -
dc.identifier.wosid 000822640900001 -
dc.identifier.scopusid 2-s2.0-85135456263 -
dc.identifier.bibliographicCitation Journal of Men's Health, v.18, no.7 -
dc.description.isOpenAccess TRUE -
dc.subject.keywordAuthor Transient receptor potential cation channel-subfamily M member 7 -
dc.subject.keywordAuthor Migration ability -
dc.subject.keywordAuthor Cell prolif -
dc.subject.keywordAuthor eration -
dc.subject.keywordAuthor Prostate cancer therapy -
dc.subject.keywordAuthor Src signaling -
dc.subject.keywordPlus ACTIVATION -
dc.subject.keywordPlus PROLIFERATION -
dc.subject.keywordPlus INCREASE -
dc.subject.keywordPlus SERUM-CALCIUM -
dc.citation.number 7 -
dc.citation.title Journal of Men's Health -
dc.citation.volume 18 -
dc.description.journalRegisteredClass scie -
dc.description.journalRegisteredClass ssci -
dc.description.journalRegisteredClass scopus -
dc.relation.journalResearchArea Public, Environmental & Occupational Health -
dc.relation.journalWebOfScienceCategory Public, Environmental & Occupational Health -
dc.type.docType Article -
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