Suppression of lung inflammation by the methanol extract of Spilanthes acmella Murray is related to differential regulation of NF-κB and Nrf2

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dc.contributor.authorK H Kim-
dc.contributor.authorE J Kim-
dc.contributor.authorM J Kwun-
dc.contributor.authorJ Y Lee-
dc.contributor.authorT T Bach-
dc.contributor.authorSang Mi Eum-
dc.contributor.authorJ Y Choi-
dc.contributor.authorS Cho-
dc.contributor.authorS J Kim-
dc.contributor.authorS I Jeong-
dc.contributor.authorM Joo-
dc.date.accessioned2018-04-19T05:18:59Z-
dc.date.available2018-04-19T05:18:59Z-
dc.date.issued2018-
dc.identifier.issn0378-8741-
dc.identifier.uri10.1016/j.jep.2018.02.011ko
dc.identifier.urihttps://oak.kribb.re.kr/handle/201005/17733-
dc.description.abstractEthnopharmacological relevance: Although Spilanthes acmella has been used to relieve inflammation, fever, pain, or infection in traditional Asian medicine, experimental evidence supporting these functions is scarce. Here, we examined an anti-inflammatory function and a possible underlying mechanism of S. acmella Murray (SAM). Materials and method: The methanol extract of SAM was fingerprinted by HPLC. C57BL/6 mice were administered with a single intratracheal (i.t.) LPS and 2 h later with a single i.t. SAM. The effect of SAM on lung inflammation was assessed by histology, semi-quantitative RT-PCR, and MPO assay of lung tissue. The effects of SAM on a pro-inflammatory factor NF-κB and an anti-inflammatory factor Nrf2 were analyzed by immunoblotting of nuclear proteins and by semi-quantitative RT-PCR analysis of mRNA of the genes governed by these transcription factors. V5-Nrf2 was precipitated by an anti-V5 antibody and the ubiquitinated V5-Nrf2 was revealed by immunoblotting of HA-tagged ubiquitin. Results: The i.t. SAM robustly diminished a neutrophilic lung inflammation induced by i.t. LPS treatment of mice. In RAW 264.7 cells, SAM suppressed the nuclear localization of NF-κB and the expression of NF-κB-dependent cytokine genes. SAM increased the level of Nrf2 in the nucleus and the expression of Nrf2-dependent genes while suppressing ubiquitination of Nrf2. Conclusion: Our results suggest that SAM can suppress a neutrophilic inflammation in mouse lungs, which is associated with suppressed NF-κB and activated Nrf2. Our results provide experimental evidence supporting the anti-inflammatory function of S. acmella-
dc.publisherElsevier-
dc.titleSuppression of lung inflammation by the methanol extract of Spilanthes acmella Murray is related to differential regulation of NF-κB and Nrf2-
dc.title.alternativeSuppression of lung inflammation by the methanol extract of Spilanthes acmella Murray is related to differential regulation of NF-κB and Nrf2-
dc.typeArticle-
dc.citation.titleJournal of Ethnopharmacology-
dc.citation.number0-
dc.citation.endPage97-
dc.citation.startPage89-
dc.citation.volume217-
dc.contributor.affiliatedAuthorSang Mi Eum-
dc.contributor.alternativeName김견하-
dc.contributor.alternativeName김은정-
dc.contributor.alternativeName권민정-
dc.contributor.alternativeName이지연-
dc.contributor.alternativeNameBach-
dc.contributor.alternativeName엄상미-
dc.contributor.alternativeName최준용-
dc.contributor.alternativeName조사연-
dc.contributor.alternativeName김상준-
dc.contributor.alternativeName정승일-
dc.contributor.alternativeName주명수-
dc.identifier.bibliographicCitationJournal of Ethnopharmacology, vol. 217, pp. 89-97-
dc.identifier.doi10.1016/j.jep.2018.02.011-
dc.subject.keywordAnti-inflammation-
dc.subject.keywordNF-B-
dc.subject.keywordNeutrophilic lung inflammation-
dc.subject.keywordNrf2-
dc.subject.keywordSpilanthes acmella Murray-
dc.subject.localantiinflammation-
dc.subject.localAntiinflammation-
dc.subject.localanti-inflammation-
dc.subject.localAnti-Inflammation-
dc.subject.localAnti-inflammation-
dc.subject.localNF-B-
dc.subject.localNeutrophilic lung inflammation-
dc.subject.localNRF2-
dc.subject.localNrf2-
dc.subject.localNrf-2-
dc.subject.localSpilanthes acmella Murray-
dc.description.journalClassY-
Appears in Collections:
Ochang Branch Institute > Division of National Bio-Infrastructure > International Biological Material Research Center > 1. Journal Articles
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