VIP modulates human macrophages phenotype via FPRL1 via activation of RhoA-GTPase and PLC pathways

Objective and design This study is aimed at uncovering the signaling pathways activated by vasoactive intestinal peptide in human macrophages Materials Human peripheral blood mononuclear cell-derived macrophages were used for the in vitro investigation of the VIP-activated signaling pathways. Method...

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Published inInflammation research Vol. 70; no. 3; pp. 309 - 321
Main Authors Harhous, Zeina, Faour, Wissam H., El Zein, Nabil
Format Journal Article
LanguageEnglish
Published Cham Springer International Publishing 01.03.2021
Springer Nature B.V
Subjects
AKT protein
Allergology
Biomedical and Life Sciences
Biomedicine
Calcium
Calcium (intracellular)
CD11b antigen
Cell activation
Cyclic AMP
Dendritic cells
Dermatology
Gelatinase B
Genotype & phenotype
Guanosine triphosphatases
Guanosine triphosphate
Hydrogen peroxide
Immunology
Inflammation
Intestine
Intracellular
Investigations
Kinases
Macrophages
MAP kinase
Neurology
Original Research Paper
Oxidative stress
Peptides
Peripheral blood
Pharmacology/Toxicology
Phenotypes
Protein kinase A
Rheumatology
RhoA protein
Roles
Signal transduction
Signaling
siRNA
Spectrometry
Vasoactive agents
Vasoactive intestinal peptide
Rho kinase
VIP
MAPK
FPRL1
Macrophage
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Summary:Objective and design This study is aimed at uncovering the signaling pathways activated by vasoactive intestinal peptide in human macrophages Materials Human peripheral blood mononuclear cell-derived macrophages were used for the in vitro investigation of the VIP-activated signaling pathways. Methods and treatment Time-course and dose–response experiments and siRNA were used in human macrophages co-challenged with various concentrations of VIP and different MAPK pharmacologic inhibitors to investigate signaling pathways activated by VIP. Flow analysis was performed to assess the levels of CD11b, CD35 and CD66. Luminescence spectrometry was used to measure the levels of the released hydrogen peroxide and the intracellular calcium levels in the media. Results Macrophages incubated with VIP showed increased phospho-AKT and phospho-ERK1/2 levels in a GTP-RhoA-GTPase-dependent manner. Similarly, VIP increased intracellular release of H 2 O 2 and calcium via PLC and GTP-RhoA-GTPase, in addition to inducing the expression of CD11b, CD35, CD66 and MMP9. Furthermore, VIP activated P38 MAPK through the cAMP/PKA pathway but was independent of both PLC and RhoA signaling. The above-mentioned VIP effects were mediated via activation of the FPRL1 receptor. Conclusion VIP/FPRL1/VPAC/GTP-RhoA-GTPase signaling modulated macrophages phenotype through activation of multiple signaling pathways including ERK1/2, AKT, P38, ROS, cAMP and calcium.
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SourceType-Scholarly Journals-1
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ISSN:1023-3830
1420-908X
DOI:10.1007/s00011-021-01436-3