Soluble Uric Acid Activates the NLRP3 Inflammasome

被引:0
作者
Tarcio Teodoro Braga
Maria Fernanda Forni
Matheus Correa-Costa
Rodrigo Nalio Ramos
Jose Alexandre Barbuto
Paola Branco
Angela Castoldi
Meire Ioshie Hiyane
Mariana Rodrigues Davanso
Eicke Latz
Bernardo S. Franklin
Alicia J. Kowaltowski
Niels Olsen Saraiva Camara
机构
[1] Laboratory of Transplantation Immunobiology,Department of Immunology
[2] Institute of Biomedical Sciences IV,Departamento de Bioquímica
[3] University of São Paulo (USP),Laboratory of Tumor Immunology Department of Immunology
[4] Institute of Innate Immunity,Department of Cellular Biology
[5] University Hospital, Institute of Biomedical Sciences
[6] University of Bonn,Division of Infectious Diseases & Immunology
[7] Instituto de Química,Department of Cancer Research and Molecular Medicine
[8] USP,Nephrology Division
[9] Institute of Biomedical Sciences IV,undefined
[10] University of São Paulo (USP),undefined
[11] University of São Paulo (USP),undefined
[12] University of Massachusetts Medical School,undefined
[13] German Center for Neurodegenerative Diseases,undefined
[14] Center of Molecular Inflammation Research,undefined
[15] Norwegian University of Science and Technology,undefined
[16] Laboratory of Clinical and Experimental Immunology,undefined
[17] Federal University of São Paulo (UNIFESP),undefined
[18] Renal Pathophysiology Laboratory (LIM16),undefined
[19] Faculty of Medicine,undefined
[20] University of São Paulo,undefined
来源
Scientific Reports | / 7卷
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摘要
Uric acid is a damage-associated molecular pattern (DAMP), released from ischemic tissues and dying cells which, when crystalized, is able to activate the NLRP3 inflammasome. Soluble uric acid (sUA) is found in high concentrations in the serum of great apes, and even higher in some diseases, before the appearance of crystals. In the present study, we sought to investigate whether uric acid, in the soluble form, could also activate the NLRP3 inflammasome and induce the production of IL-1β. We monitored ROS, mitochondrial area and respiratory parameters from macrophages following sUA stimulus. We observed that sUA is released in a hypoxic environment and is able to induce IL-1β release. This process is followed by production of mitochondrial ROS, ASC speck formation and caspase-1 activation. Nlrp3−/− macrophages presented a protected redox state, increased maximum and reserve oxygen consumption ratio (OCR) and higher VDAC protein levels when compared to WT and Myd88−/− cells. Using a disease model characterized by increased sUA levels, we observed a correlation between sUA, inflammasome activation and fibrosis. These findings suggest sUA activates the NLRP3 inflammasome. We propose that future therapeutic strategies for renal fibrosis should include strategies that block sUA or inhibit its recognition by phagocytes.
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