Anti-inflammatory effects of Perilla frutescens in activated human neutrophils through two independent pathways: Src family kinases and Calcium

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作者
Chun-Yu Chen
Yann-Lii Leu
Yu Fang
Chwan-Fwu Lin
Liang-Mou Kuo
Wei-Che Sung
Yung-Fong Tsai
Pei-Jen Chung
Ming-Chung Lee
Yu-Ting Kuo
Hsuan-Wu Yang
Tsong-Long Hwang
机构
[1] Graduate Institute of Natural Products,Department of Anesthesiology
[2] School of Traditional Chinese Medicine,Department of Cosmetic Science
[3] College of Medicine,Division of General Surgery, Department of Surgery
[4] Chang Gung University,Department of Cosmetic Science and Research Center for Industry of Human Ecology
[5] Graduate Institute of Clinical Medical Sciences,undefined
[6] College of Medicine,undefined
[7] Chang Gung University,undefined
[8] Chang Gung Memorial Hospital,undefined
[9] Chang Gung University of Science and Technology,undefined
[10] Chang Gung Memorial Hospital,undefined
[11] Brion Research Institute of Taiwan,undefined
[12] Chinese Herbal Medicine Research Team,undefined
[13] Healthy Aging Research Center,undefined
[14] Chang Gung University,undefined
[15] Chang Gung University of Science and Technology,undefined
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摘要
The leaves of Perilla frutescens (L.) Britt. have been traditionally used as an herbal medicine in East Asian countries to treat a variety diseases. In this present study, we investigated the inhibitory effects of P. frutescens extract (PFE) on N-formyl-Met-Leu-Phe (fMLF)-stimulated human neutrophils and the underlying mechanisms. PFE (1, 3 and 10 μg/ml) inhibited superoxide anion production, elastase release, reactive oxygen species formation, CD11b expression and cell migration in fMLF-activated human neutrophils in dose-dependent manners. PFE inhibited fMLF-induced phosphorylation of the Src family kinases (SFKs), Src (Tyr416) and Lyn (Tyr396) and reduced their enzymatic activities. Both PFE and PP2 (a selective inhibitor of SFKs) reduced the phosphorylation of Burton’s tyrosine kinases (Tyr223) and Vav (Tyr174) in fMLF-activated human neutrophils. Additionally, PFE decreased intracellular Ca2+ levels ([Ca2+]i), whereas PP2 prolonged the time required for [Ca2+]i to return to its basal level. Our findings indicated that PFE effectively regulated the inflammatory activities of fMLF-activated human neutrophils. The anti-inflammatory effects of PFE on activated human neutrophils were mediated through two independent signaling pathways involving SFKs (Src and Lyn) and mobilization of intracellular Ca2+.
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