Article(id=1218551213088493706, tenantId=1146029695717560320, journalId=1189982191388893191, issueId=1218551209271677657, articleNumber=null, orderNo=null, doi=10.16438/j.0513-4870.2018-0713, pmid=null, cstr=null, oa=null, hot=null, price=null, onlineType=0, articleFormat=0, articleType=null, articleTypeStr=research-article, receivedDate=1533484800000, receivedDateStr=2018-08-06, revisedDate=1535817600000, revisedDateStr=2018-09-02, acceptedDate=null, acceptedDateStr=null, onlineDate=1768454848787, onlineDateStr=2026-01-15, pubDate=1544544000000, pubDateStr=2018-12-12, doiRegisterDate=null, doiRegisterDateStr=null, onlineIssueDate=1768454848787, onlineIssueDateStr=2026-01-15, onlineJustAcceptDate=null, onlineJustAcceptDateStr=null, onlineFirstDate=null, onlineFirstDateStr=null, sourceXml=null, magXml=null, createTime=1768454848787, creator=13701087609, updateTime=1768454848787, updator=13701087609, issue=Issue{id=1218551209271677657, tenantId=1146029695717560320, journalId=1189982191388893191, year='2018', volume='53', issue='12', pageStart='1943', pageEnd='2134', issueExtLink='null', onlineDate='null', pubDate='null', beforeIssueId=null, nextIssueId=null, price=null, status=1, issueComplete=1, articleOrder=1, issueType=-1, specialIssue=null, createTime=1768454847877, creator=13701087609, updateTime=1768457192749, updator=13701087609, preIssue=null, nextIssue=null, ext={EN=IssueExt(id=1218561044428017831, tenantId=1146029695717560320, journalId=1189982191388893191, issueId=1218551209271677657, language=EN, specialIssueTitle=, coverIllustrator=null, specialIssueEditor=, specialIssueAbout=), CN=IssueExt(id=1218561044428017832, tenantId=1146029695717560320, journalId=1189982191388893191, issueId=1218551209271677657, language=CN, specialIssueTitle=, coverIllustrator=null, specialIssueEditor=, specialIssueAbout=)}, issueFiles=null}, startPage=2050, endPage=2056, ext={EN=ArticleExt(id=1218551213742805206, articleId=1218551213088493706, tenantId=1146029695717560320, journalId=1189982191388893191, language=EN, title=Inhibitory effect and mechanism of licochalcone A on NLRP3 inflammasome, columnId=1218551213583421639, journalTitle=Acta Pharmaceutica Sinica, columnName=Pharmacology, runingTitle=null, highlight=null, articleAbstract=

Lipopolysaccharide (LPS)-induced bone marrow-derived macrophages (BMDMs), treated with licochalcone A (LCA) and retreated with inflammasome inducers respectively (ATP and nigericin), were used to construct the inflammasome model of NLRP3 (NOD-like receptor family, pyrin domain containing 3), to investigate the inhibitory effect and the molecular mechanism of LCA on the activity of NLRP3 inflammasome. The secretion of mature interleukin (IL)-1β, tumor necrosis factor-α (TNF-α) and caspase-1 in the supernatants were analyzed by ELISA and the Caspase-Glo^® 1 Inflammasome Assay. Supernatants and cell lysates were analyzed for the expression of pro-caspase-1, pro-IL-1β, ASC, NLRP3, IL-1β, caspase-1 by immunoblotting. The study shows that LCA inhibited the activity of caspase-1 and the secretion of IL-1β, and suppressed the activity of NLRP3 inflammasome. There was also slight inhibition of NLRC4 inflammasome induced by Lfn-Flic, but no effect on poly(dA:dT)-induced the absent in melanoma 2 (AIM2) inflammasome. Western blot showed that LCA had no effect on the protein expression of NLRP3 and pro-IL-1β, which was mediated by NF-κB pathway. In summary, LCA can inhibit the cleavage of pro-caspase-1 and suppress the secretion of IL-1β to reduce the inflammation response. The study was carried out under the approval of the Scientific Investigation Board of 302 Hospital of PLA.

, correspAuthors=Zhao-fang BAI, Xiao-he XIAO, authorNote=null, correspAuthorsNote=null, copyrightStatement=Copyright ©2018 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=Shu-bin FU, Guang XU, Yuan GAO, Zhi-lei WANG, Nan QIN, Hui-min LIU, Zhao-fang BAI, Xiao-he XIAO), CN=ArticleExt(id=1218551215487635844, articleId=1218551213088493706, tenantId=1146029695717560320, journalId=1189982191388893191, language=CN, title=甘草查尔酮A对NLRP3炎症小体的调控作用及机制初探, columnId=1190335348896011050, journalTitle=药学学报, columnName=研究论文, runingTitle=null, highlight=null, articleAbstract=

利用小鼠原代骨髓巨噬细胞（bone marrow-derived macrophages，BMDMs）构建NOD（nucleotide binding oligomerization domain）样受体家族3（NOD-like receptors，NLRP3）炎症小体活化模型，探讨甘草查尔酮A（licochalcone A，LCA）对NLRP3炎症小体的调控作用及初步机制。脂多糖（lipopolysaccharide，LPS）预处理BMDMs细胞后给予LCA，分别再给予三磷酸腺苷（adenosine triphosphate，ATP）和尼日利亚菌素（nigericin）刺激构建NLRP3炎症小体活化模型，采用Caspase-Glo^® 1 Inflammasome Assay和ELISA检测细胞培养上清液中半胱氨酸天冬氨酸特异蛋白酶1（caspase-1）的活性、白细胞介素（interleukin，IL）-1β和肿瘤坏死因子-α（tumor necrosis factor-α，TNF-α）分泌；通过免疫印迹法（Western blot）检测细胞上清中的成熟IL-1β、caspase-1的产生及细胞裂解液中NLRP3、凋亡相关斑点样蛋白（apoptosis-associated speck-like protein，ASC）和pro-caspase-1、pro-IL-1β的表达。Caspase-Glo^® 1 Inflammasome Assay和ELISA结果表明，LCA能显著抑制ATP和nigericin诱导的NLRP3炎症小体组成蛋白pro-caspase-1和pro-IL-1β剪切活化，同时对细菌鞭毛蛋白（Lfn-Flic）诱导的NOD样受体家族半胱天冬酶激活募集结构域4（NOD-like receptor containing a caspase activating and recruitment domain 4，NLRC4）炎症小体活性也具轻微抑制作用，但是对poly（dA：dT）诱导的黑色素瘤缺乏因子2（the absent in melanoma 2，AIM2）炎症小体活化无影响。免疫印迹法检测显示LCA对NF-κB介导的NLRP3炎症小体组成蛋白NLRP3和pro-IL-1β表达无影响。综上，研究表明LCA可通过抑制pro-caspase-1剪切，阻断caspase p20介导的pro-IL-1β的剪切成熟，最终抑制NLRP3炎症小体介导免疫炎症反应。本研究在中国人民解放军第302医院伦理委员会审批下进行，为甘草及LCA防治NLRP3炎症小体相关疾病提供了依据。

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Gastroenterology, 2017, 152:S886., articleTitle=null, refAbstract=null), Reference(id=1218970822337806414, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218551213088493706, doi=null, pmid=null, pmcid=null, year=null, volume=null, issue=null, pageStart=null, pageEnd=null, url=null, language=null, rfNumber=[27], rfOrder=26, authorNames=null, journalName=null, refType=null, unstructuredReference=Wang YY, Li HT, Lu Y, et al. Protective effects of glycyrrhizic acid against lupus nephritis in MRL/lpr mice[J]. J South Med Univ (南方医科大学学报), 2017, 37:957-961., articleTitle=null, refAbstract=null), Reference(id=1218970822438469723, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218551213088493706, doi=null, pmid=null, pmcid=null, year=null, volume=null, issue=null, pageStart=null, pageEnd=null, url=null, language=null, rfNumber=[28], rfOrder=27, authorNames=null, journalName=null, refType=null, unstructuredReference=Sutterwala FS, Haasken S, Cassel SL. Mechanism of NLRP3 inflammasome activation[J]. Ann N Y Acad Sci, 2014, 1319:82-95., articleTitle=null, refAbstract=null), Reference(id=1218970822539133030, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218551213088493706, doi=null, pmid=null, pmcid=null, year=null, volume=null, issue=null, pageStart=null, pageEnd=null, url=null, language=null, rfNumber=[29], rfOrder=28, authorNames=null, journalName=null, refType=null, unstructuredReference=Bauernfeind FG, Horvath G, Stutz A, et al. Cutting edge:NF-κB activating pattern recognition and cytokine receptors license NLRP3 inflammasome activation by regulating NLRP3 expression[J]. J Immunol, 2009, 183:787-791., articleTitle=null, refAbstract=null), Reference(id=1218970822643990639, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218551213088493706, doi=null, pmid=null, pmcid=null, year=null, volume=null, issue=null, pageStart=null, pageEnd=null, url=null, language=null, rfNumber=[30], rfOrder=29, authorNames=null, journalName=null, refType=null, unstructuredReference=Tsutsui H, Imamura M, Fujimoto J, et al. The TLR4/TRIF-mediated activation of NLRP3 inflammasome underlies endotoxin-induced liver injury in mice[J]. 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A: LCA structure; B: Effect of LCA on cell viability in immortalized bone marrow-derived macrophages (iBMDMs). The cells were treated with various of concentrations of LCA for 12 h. n = 5, $\overline{x}±s$. C: Effect of LCA on cell viability in bone marrow-derived macrophages (BMDMs). The cells were treated with various of concentrations of LCA for 24 h. n = 3, $\overline{x}±s$. ^**P < 0.01, ^***P < 0.001 vs control group

, figureFileSmall=+mQTFXC12S93GcstnT0+Ew==, figureFileBig=+a6eiGl01CDO9lgbb471yA==, tableContent=null), ArticleFig(id=1218970814951637517, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218551213088493706, language=EN, label=null, caption=null, figureFileSmall=/9hxy5dBcdPlz0A+zDff1Q==, figureFileBig=5zjN3jGKlY+W5LItMtkMqg==, tableContent=null), ArticleFig(id=1218970815106826777, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218551213088493706, language=CN, label=Figure 2, caption=

A: Western blot was used to assess the expression levels of indicated proteins in culture supernatants (Sup.) and cell lysates (Lys.). Lamin B was used as a loading control for cell lysates. Coomassie blue staining was provided as the loading control for the supernatants. B: The activity of caspase-1 was analyzed in the supernatant of BMDMs by the Caspase-Glo^® 1 Inflammasome Assay. RLU, recombinant luciferase, which is proportional to caspase-1 activity. C, D: The secretion of IL-1β and TNF-α was measured in the supernatant of BMDMs by ELISA. n = 3, $\overline{x}±s$. ^*P < 0.05, ^**P < 0.01, ^***P < 0.001 vs LPS+ATP group; ^###P < 0.001 vs control (DMSO) group. ns: Nonsignificant

, figureFileSmall=/9hxy5dBcdPlz0A+zDff1Q==, figureFileBig=5zjN3jGKlY+W5LItMtkMqg==, tableContent=null), ArticleFig(id=1218970815253627435, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218551213088493706, language=EN, label=null, caption=null, figureFileSmall=fG3G7k6vRCfXuapkKfyNJA==, figureFileBig=7Kh33AB1Xxm0/G/fYepDPw==, tableContent=null), ArticleFig(id=1218970815358485045, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218551213088493706, language=CN, label=Figure 3, caption=

A: Western blot was used to assess the expression levels of indicated proteins in culture supernatants and cell lysates. Lamin B was used as a loading control for cell lysates. Coomassie blue staining was provided as the loading control for the supernatants. B: The activity of caspase-1 was analyzed in the supernatant of BMDMs by the Caspase-Glo^® 1 Inflammasome Assay. RLU, recombinant luciferase, which is proportional to caspase-1 activity. C, D: The secretion of IL-1β and TNF-α was measured in the supernatant of BMDMs by ELISA. n = 3, $\overline{x}±s$. ^**P < 0.01, ^***P < 0.001 vs LPS+Nigericin group; ^###P < 0.001 vs control (DMSO) group

, figureFileSmall=fG3G7k6vRCfXuapkKfyNJA==, figureFileBig=7Kh33AB1Xxm0/G/fYepDPw==, tableContent=null), ArticleFig(id=1218970815471731271, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218551213088493706, language=EN, label=null, caption=null, figureFileSmall=m2ExmA6xg8yv5DRlPK9lUw==, figureFileBig=qaiZtzYtZNTza/YfQbIHpA==, tableContent=null), ArticleFig(id=1218970815589171796, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218551213088493706, language=CN, label=Figure 4, caption=

A: Western blot was used to assess the expression levels of indicated proteins in culture supernatants and cell lysates. Lamin B was used as a loading control for cell lysates. Coomassie blue staining was provided as the loading control for the supernatants. B: The activity of caspase-1 was analyzed in the supernatant of BMDMs by the Caspase-Glo^® 1 Inflammasome Assay. RLU, recombinant luciferase, which is proportional to caspase-1 activity. C, D: The secretion of IL-1β and TNF-α was measured in the supernatant of BMDMs by ELISA. n = 3, $\overline{x}±s$. ^*P < 0.05, ^***P < 0.001 vs control (DMSO) group. NLRC4: NOD-like receptor containing a caspase activating and recruitment domain 4; AIM2: The absent in melanoma 2

, figureFileSmall=m2ExmA6xg8yv5DRlPK9lUw==, figureFileBig=qaiZtzYtZNTza/YfQbIHpA==, tableContent=null), ArticleFig(id=1218970815731778152, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218551213088493706, language=EN, label=null, caption=null, figureFileSmall=dCL+Tn0b32JmQkp6R7Bt/Q==, figureFileBig=msW7sB+fMkM4uG+11+W/Aw==, tableContent=null), ArticleFig(id=1218970815891161723, tenantId=1146029695717560320, journalId=1189982191388893191, articleId=1218551213088493706, language=CN, label=Figure 5, caption=

LCA had no effect on LPS-induced NLRP3, pro-IL-1β expression when BMDMs were treated with LCA for 30 min before 3 h LPS stimulation. The results showed that the inhibitory activity of LCA on NLRP3 inflammasome was not dependent on NF-κB pathway

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