Article(id=1218263312534524249, tenantId=1146029695717560320, journalId=1189982191388893191, issueId=1218263310198296916, articleNumber=null, orderNo=null, doi=10.16438/j.0513-4870.2016-1003, pmid=null, cstr=null, oa=null, hot=null, price=null, onlineType=0, articleFormat=0, articleType=null, articleTypeStr=research-article, receivedDate=1476633600000, receivedDateStr=2016-10-17, revisedDate=1479744000000, revisedDateStr=2016-11-22, acceptedDate=null, acceptedDateStr=null, onlineDate=1768386207945, onlineDateStr=2026-01-14, pubDate=1484150400000, pubDateStr=2017-01-12, doiRegisterDate=null, doiRegisterDateStr=null, onlineIssueDate=1768386207945, onlineIssueDateStr=2026-01-14, onlineJustAcceptDate=null, onlineJustAcceptDateStr=null, onlineFirstDate=null, onlineFirstDateStr=null, sourceXml=null, magXml=null, createTime=1768386207945, creator=13701087609, updateTime=1768386207945, updator=13701087609, issue=Issue{id=1218263310198296916, tenantId=1146029695717560320, journalId=1189982191388893191, year='2017', volume='52', issue='1', pageStart='1', pageEnd='179', issueExtLink='null', onlineDate='null', pubDate='null', beforeIssueId=null, nextIssueId=null, price=null, status=1, issueComplete=1, articleOrder=1, issueType=-1, specialIssue=null, createTime=1768386207389, creator=13701087609, updateTime=1768386435964, updator=13701087609, preIssue=null, nextIssue=null, ext={EN=IssueExt(id=1218264268965856067, tenantId=1146029695717560320, journalId=1189982191388893191, issueId=1218263310198296916, language=EN, specialIssueTitle=, coverIllustrator=null, specialIssueEditor=, specialIssueAbout=), CN=IssueExt(id=1218264268965856068, tenantId=1146029695717560320, journalId=1189982191388893191, issueId=1218263310198296916, language=CN, specialIssueTitle=, coverIllustrator=null, specialIssueEditor=, specialIssueAbout=)}, issueFiles=null}, startPage=51, endPage=57, ext={EN=ArticleExt(id=1218263313767649642, articleId=1218263312534524249, tenantId=1146029695717560320, journalId=1189982191388893191, language=EN, title=Regulation of P-glycoprotein gene expression by PKC/NF-
κB-PXR signaling pathway, columnId=1218263312677130587, journalTitle=Acta Pharmaceutica Sinica, columnName=SPECIAL REPORTS, runingTitle=null, highlight=null, articleAbstract=
P-glycoprotein (P-gp), an ATP binding cassette protein, plays a major role in efflux transport of drugs and xenobiotics due to its abundant expression on several barriers. This study aimed to investigate the potential role of PKC/NF-κB-PXR signaling pathway in modulation of P-gp gene expression in human colon adenocarcinoma LS174T. The effect of PMA on MDR1 luciferase activity was investigated by PXR-MDR1 dual luciferase reporter gene assay. Real-time qPCR assay and Western blot analysis were used to study the gene expression of P-gp and NF-κB, respectively. Compared to the vehicle-treated group, PMA statistically decreased P-gp luciferase activity, mRNA expression and protein expression. Moreover, PMA treatment yielded a significant and dose-dependent increase in RelA/p65 translocation to nucleus. Meanwhile, a remarkable increase of the pho-IκBα status was observed in LS174T cells after treatment with PMA (1-100 nmol·L-1). In addition, knockdown of PKCα, NF-κB or PXR can significantly attenuate PMA-induced P-gp suppression.These results suggested that PKC/NF-κB-PXR signaling pathway might play crucial roles in modulation of P-gp gene expression.
, correspAuthors=Hui-chang BI, authorNote=null, correspAuthorsNote=null, copyrightStatement=Copyright © 2016 ACTA PHARMACEUTICA SINICA All rights reserved., copyrightOwner=null, extLink=null, articleAbsUrl=null, sourceXml=null, magXml=null, pdfUrl=null, pdf=null, pdfFileSize=null, pdfExtLink=null, richHtmlUrl=null, mobilePdfUrl=null, reviewReport=null, pdfFirstPage=null, abstractGraph=null, abstractGraphContent=null, abstractVideo=null, citation=null, cebUrl=null, magXmlContent=null, mapNumber=null, authorCompany=null, fund=null, authors=null, authorsList=Yu-hua LI, Ling HUANG, Xiao-hua WEI, Jin-hua WEN, Guo-ping ZHONG, Min HUANG, Hui-chang BI), CN=ArticleExt(id=1218263316875629011, articleId=1218263312534524249, tenantId=1146029695717560320, journalId=1189982191388893191, language=CN, title=PKC/NF-
κB-PXR信号通路对P-糖蛋白基因表达的调控研究, columnId=1218263312865874270, journalTitle=药学学报, columnName=专题报道, runingTitle=null, highlight=null, articleAbstract=
P-糖蛋白(P-gp)是ABC(ATP binding cassette)转运体家族重要成员,也是药物在机体内转运的重要载体。本文考察PKC/NF-κB-PXR信号途径对LS174T细胞中P-gp基因表达的调控作用。运用孕甾烷X受体(PXR)-MDR1双荧光报告基因实验探究PKC激动剂佛波酯(PMA)对LS174T细胞中MDR1荧光素酶活性的影响;分别采用real-time qPCR和Western blot检测PMA对LS174T细胞中P-gp mRNA表达、蛋白表达及NF-κB通路相关蛋白的影响。结果表明,PKC激动剂PMA能明显抑制PXR介导的P-gp荧光素酶活性、mRNA和蛋白表达,并能显著性增加胞内RelA/p65的核转位。此外,siRNA干扰实验结果显示,PKCα siRNA、RelA siRNA或PXR siRNA干扰均可显著削弱PMA对P-gp基因表达的下调作用。因此,PKC激动剂能显著抑制PXR介导的P-gp基因表达并伴随NF-κB激活,提示PKC/NF-κB-PXR信号通路对P-gp基因表达具有重要的调控作用。
, correspAuthors=毕惠嫦, authorNote=null, correspAuthorsNote=
, copyrightStatement=版权所有 © 《药学学报》编辑部 2017, copyrightOwner=null, extLink=null, articleAbsUrl=null, sourceXml=wfm7BeQSNnMDrfGpCRDtaw==, magXml=NFxFBxNWaxsrzBB5O5R38Q==, pdfUrl=null, pdf=gNeMfLuxykRceDz9P1Be6w==, pdfFileSize=4621283, pdfExtLink=null, richHtmlUrl=null, mobilePdfUrl=null, reviewReport=null, pdfFirstPage=null, abstractGraph=97QmcDTA5zTcNHw+Nq/h6g==, abstractGraphContent=null, abstractVideo=null, citation=null, cebUrl=null, magXmlContent=CQxxZ3CiuOAweO+2cLMOAA==, mapNumber=null, authorCompany=null, fund=null, authors=null, authorsList=黎玉华, 黄凌, 魏筱华, 温金华, 钟国平, 黄民, 毕惠嫦)}, authors=[Author(id=1218968385371689915, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218263312534524249, orderNo=0, firstName=null, middleName=null, lastName=null, nameCn=null, orcid=null, stid=null, country=null, authorPic=null, dead=0, email=null, emailSecond=null, emailThird=null, correspondingAuthor=0, authorType=1, ext={EN=AuthorExt(id=1218968385535267796, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218263312534524249, authorId=1218968385371689915, language=EN, stringName=Yu-hua LI, firstName=Yu-hua, middleName=null, lastName=LI, prefix=null, suffix=null, authorComment=null, nameInitials=null, affiliation=null, department=null, xref=
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κB), Keyword(id=1218968393949041060, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218263312534524249, language=CN, orderNo=3, keyword=孕甾烷X受体), Keyword(id=1218968394037121457, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218263312534524249, language=CN, orderNo=4, keyword=P-糖蛋白), Keyword(id=1218968394154561981, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218263312534524249, language=CN, orderNo=5, keyword=基因表达)], refs=[Reference(id=1218968396310434440, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218263312534524249, doi=null, pmid=null, pmcid=null, year=null, volume=null, issue=null, pageStart=null, pageEnd=null, url=null, language=null, rfNumber=[1], rfOrder=0, authorNames=null, journalName=null, refType=null, unstructuredReference=Higgins CF. ABC transporters:from microorganisms to man[J]. 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Activation of endogenous phorbol ester-dependent PKC signaling induces tk-MDR1-Luc reporter gene activity in LS174T cells. Five hour post-transfection, LS174T cells were treated with the indicated concentrations (nmol·L-1) of PMA (phorbol 12-myristate 13-acetate) or PKC-inactive 4α-PMA in the presence and absence of rifampicin (Rif, 10 μmol·L-1) for 24 h. The data presented are the mean ± S.D. of triplicates (n = 3) and are expressed as reporter gene activity; *P < 0.05 vs Control
, figureFileSmall=s0Iu2rd6t4AUFzuU8jrhrg==, figureFileBig=7F11GVCPK4VdN5Gq5GEB3w==, tableContent=null), ArticleFig(id=1218968394804679145, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218263312534524249, language=EN, label=null, caption=null, figureFileSmall=GdtRo5oSokmqqtqGgXpI6g==, figureFileBig=L8XGamUo5a1cUc+kUw7ISQ==, tableContent=null), ArticleFig(id=1218968394930508278, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218263312534524249, language=CN, label=Figure 2, caption=
The effect of 4α-PMA and PMA on the mRNA expression (A) and protein expression (B) of P-gp in LS174T cell. The cells were treated with vehicle controls (0.1% DMSO); 100 nmol·L-1 4α-PMA; 1, 10, 100, 500 nmol·L-1 PMA for 48 h, respectively. Total RNA and proteins were harvested. P-gp mRNA levels were analyzed by real-time PCR. Proteins were analyzed by Western blot. Expression of tested genes was normalized against that of GAPDH. The effect of PMA on the P-gp expression levels is presented as percentage expression compared to the vehicle group. The data presented are the mean ± S.D. of triplicates (n = 3) ; *P < 0.05 vs Control
, figureFileSmall=GdtRo5oSokmqqtqGgXpI6g==, figureFileBig=L8XGamUo5a1cUc+kUw7ISQ==, tableContent=null), ArticleFig(id=1218968395081503238, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218263312534524249, language=EN, label=null, caption=null, figureFileSmall=tDdwy9+FnkDeV7NzbMIPgA==, figureFileBig=K4JEfue6sitq+W8uSe1b7Q==, tableContent=null), ArticleFig(id=1218968395215720980, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218263312534524249, language=CN, label=Figure 3, caption=
Effect of PMA on the NF-κB signaling pathway in LS174T cells. The cells were treated with vehicle control (0.1% DMSO) or PMA at concentrations of 1, 10, 100, 500 nmol·L-1 for 48 h. Cytoplasmic and nuclear extracts were prepared. The levels of NF-κB (p65/RelA) in the nucleus, the phosphorylation of IKKα/β, and the phosphorylation of IκBα and the cytosolic IκBα levels were determined by Western blot. Immunoreactive proteins were visualized using an ECL method. The data that are shown represented three independent experiments
, figureFileSmall=tDdwy9+FnkDeV7NzbMIPgA==, figureFileBig=K4JEfue6sitq+W8uSe1b7Q==, tableContent=null), ArticleFig(id=1218968395362521637, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218263312534524249, language=EN, label=null, caption=null, figureFileSmall=zJ2yHR9+1wk+DASIPvov2g==, figureFileBig=QLDJiIlLRCY4UZV9nMLW/w==, tableContent=null), ArticleFig(id=1218968395496739384, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218263312534524249, language=CN, label=Figure 4, caption=
The role of PKCα in the regulation of P-gp (A) and NF-κB (B, C) due to activation of the PKC. LS174T cells were transfected with PKCα siRNA for 5 h. The cells were treated with vehicle control (0.1% DMSO); 100 nmol·L-1 4α-PMA; 1, 10 and 100 nmol·L-1 PMA for 48 h, respectively. Proteins were harvested and fractionated through 8% SDS-PAGE, transferred to PVDF filters, and incubated with primary antibodies. Immuno-reactive proteins were visualized using an ECL method
, figureFileSmall=zJ2yHR9+1wk+DASIPvov2g==, figureFileBig=QLDJiIlLRCY4UZV9nMLW/w==, tableContent=null), ArticleFig(id=1218968395639345731, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218263312534524249, language=EN, label=null, caption=null, figureFileSmall=sLYT2NMn1Aryb3AKeZ0KvA==, figureFileBig=7WfYrejnPLJUdpszF3eoZw==, tableContent=null), ArticleFig(id=1218968395786146388, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218263312534524249, language=CN, label=Figure 5, caption=
The roles of RelA (A, B) and PXR (C, D) in the regulation of P-gp due to activation of the PKC. LS174T cells were transfected with RelA siRNA or PXR siRNA for 5 h. The cells were treated with vehicle control (0.1% DMSO); 100 nmol·L-1 4α-PMA; 1, 10 and 100 nmol·L-1 PMA for 48 h, respectively. Total RNA and proteins were harvested. P-gp mRNA levels were analyzed by real-time PCR. Proteins were analyzed by Western blot. Expression of tested genes was normalized against that of GAPDH. The effect of PMA on the P-gp expression levels is presented as percentage expression compared to control vehicle-treated cells. The data presented are the mean ± S.D. of triplicates (n = 3) ; *P < 0.05, **P < 0.01, ***P < 0.001 vs Control
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