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Conditional deletion of caspase-8 in macrophages alters macrophage activation in a RIPK-dependent manner
by
Cuda, Carla M.
, Budinger, G. R. Scott
, Khare, Sonal
, Homan, Philip J.
, Stehlik, Christian
, Hutcheson, Jack
, Dorfleutner, Andrea
, Misharin, Alexander V.
, Tsai, FuNien
, Archer, Amy M.
, Perlman, Harris
, Saber, Rana
, Haines, G. Kenneth
in
Analysis
/ Animals
/ Antigens, Differentiation - immunology
/ Antigens, Differentiation - metabolism
/ Antigens, Ly - immunology
/ Antigens, Ly - metabolism
/ Apoptosis
/ Arthritis
/ B7-2 Antigen - immunology
/ B7-2 Antigen - metabolism
/ Blotting, Western
/ Caspase 8 - genetics
/ Caspase 8 - immunology
/ Caspase 8 - metabolism
/ CD11b Antigen - immunology
/ CD11b Antigen - metabolism
/ Cells, Cultured
/ Enzymes
/ Female
/ Flow Cytometry
/ Genetic aspects
/ Inflammation - genetics
/ Inflammation - immunology
/ Inflammation - metabolism
/ Macrophage Activation - immunology
/ Macrophages
/ Macrophages - enzymology
/ Macrophages - immunology
/ Macrophages - metabolism
/ Medicine
/ Medicine & Public Health
/ Mice, Inbred C57BL
/ Mice, Knockout
/ Mice, Transgenic
/ Muramidase - genetics
/ Muramidase - immunology
/ Muramidase - metabolism
/ Myeloid Cells - enzymology
/ Myeloid Cells - immunology
/ Myeloid Cells - metabolism
/ Orthopedics
/ Receptor-Interacting Protein Serine-Threonine Kinases - genetics
/ Receptor-Interacting Protein Serine-Threonine Kinases - immunology
/ Receptor-Interacting Protein Serine-Threonine Kinases - metabolism
/ Research Article
/ Rheumatology
/ Spleen - immunology
/ Spleen - metabolism
/ Spleen - pathology
/ Toll-Like Receptors - immunology
/ Toll-Like Receptors - metabolism
2015
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Conditional deletion of caspase-8 in macrophages alters macrophage activation in a RIPK-dependent manner
by
Cuda, Carla M.
, Budinger, G. R. Scott
, Khare, Sonal
, Homan, Philip J.
, Stehlik, Christian
, Hutcheson, Jack
, Dorfleutner, Andrea
, Misharin, Alexander V.
, Tsai, FuNien
, Archer, Amy M.
, Perlman, Harris
, Saber, Rana
, Haines, G. Kenneth
in
Analysis
/ Animals
/ Antigens, Differentiation - immunology
/ Antigens, Differentiation - metabolism
/ Antigens, Ly - immunology
/ Antigens, Ly - metabolism
/ Apoptosis
/ Arthritis
/ B7-2 Antigen - immunology
/ B7-2 Antigen - metabolism
/ Blotting, Western
/ Caspase 8 - genetics
/ Caspase 8 - immunology
/ Caspase 8 - metabolism
/ CD11b Antigen - immunology
/ CD11b Antigen - metabolism
/ Cells, Cultured
/ Enzymes
/ Female
/ Flow Cytometry
/ Genetic aspects
/ Inflammation - genetics
/ Inflammation - immunology
/ Inflammation - metabolism
/ Macrophage Activation - immunology
/ Macrophages
/ Macrophages - enzymology
/ Macrophages - immunology
/ Macrophages - metabolism
/ Medicine
/ Medicine & Public Health
/ Mice, Inbred C57BL
/ Mice, Knockout
/ Mice, Transgenic
/ Muramidase - genetics
/ Muramidase - immunology
/ Muramidase - metabolism
/ Myeloid Cells - enzymology
/ Myeloid Cells - immunology
/ Myeloid Cells - metabolism
/ Orthopedics
/ Receptor-Interacting Protein Serine-Threonine Kinases - genetics
/ Receptor-Interacting Protein Serine-Threonine Kinases - immunology
/ Receptor-Interacting Protein Serine-Threonine Kinases - metabolism
/ Research Article
/ Rheumatology
/ Spleen - immunology
/ Spleen - metabolism
/ Spleen - pathology
/ Toll-Like Receptors - immunology
/ Toll-Like Receptors - metabolism
2015
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Conditional deletion of caspase-8 in macrophages alters macrophage activation in a RIPK-dependent manner
by
Cuda, Carla M.
, Budinger, G. R. Scott
, Khare, Sonal
, Homan, Philip J.
, Stehlik, Christian
, Hutcheson, Jack
, Dorfleutner, Andrea
, Misharin, Alexander V.
, Tsai, FuNien
, Archer, Amy M.
, Perlman, Harris
, Saber, Rana
, Haines, G. Kenneth
in
Analysis
/ Animals
/ Antigens, Differentiation - immunology
/ Antigens, Differentiation - metabolism
/ Antigens, Ly - immunology
/ Antigens, Ly - metabolism
/ Apoptosis
/ Arthritis
/ B7-2 Antigen - immunology
/ B7-2 Antigen - metabolism
/ Blotting, Western
/ Caspase 8 - genetics
/ Caspase 8 - immunology
/ Caspase 8 - metabolism
/ CD11b Antigen - immunology
/ CD11b Antigen - metabolism
/ Cells, Cultured
/ Enzymes
/ Female
/ Flow Cytometry
/ Genetic aspects
/ Inflammation - genetics
/ Inflammation - immunology
/ Inflammation - metabolism
/ Macrophage Activation - immunology
/ Macrophages
/ Macrophages - enzymology
/ Macrophages - immunology
/ Macrophages - metabolism
/ Medicine
/ Medicine & Public Health
/ Mice, Inbred C57BL
/ Mice, Knockout
/ Mice, Transgenic
/ Muramidase - genetics
/ Muramidase - immunology
/ Muramidase - metabolism
/ Myeloid Cells - enzymology
/ Myeloid Cells - immunology
/ Myeloid Cells - metabolism
/ Orthopedics
/ Receptor-Interacting Protein Serine-Threonine Kinases - genetics
/ Receptor-Interacting Protein Serine-Threonine Kinases - immunology
/ Receptor-Interacting Protein Serine-Threonine Kinases - metabolism
/ Research Article
/ Rheumatology
/ Spleen - immunology
/ Spleen - metabolism
/ Spleen - pathology
/ Toll-Like Receptors - immunology
/ Toll-Like Receptors - metabolism
2015
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Conditional deletion of caspase-8 in macrophages alters macrophage activation in a RIPK-dependent manner
Journal Article
Conditional deletion of caspase-8 in macrophages alters macrophage activation in a RIPK-dependent manner
2015
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Overview
Introduction
Although caspase-8 is a well-established initiator of apoptosis and suppressor of necroptosis, recent evidence suggests that this enzyme maintains functions beyond its role in cell death. As cells of the innate immune system, and in particular macrophages, are now at the forefront of autoimmune disease pathogenesis, we examined the potential involvement of caspase-8 within this population.
Methods
Cre
LysM
Casp8
fl/fl
mice were bred via a cross between
Casp8
fl/fl
mice and
Cre
LysM
mice, and
RIPK3
−/−
Cre
LysM
Casp8
fl/fl
mice were generated to assess the contribution of receptor-interacting serine-threonine kinase (RIPK)3. Immunohistochemical and immunofluorescence analyses were used to examine renal damage. Flow cytometric analysis was employed to characterize splenocyte distribution and activation.
Cre
LysM
Casp8
fl/fl
mice were treated with either Toll-like receptor (TLR) agonists or oral antibiotics to assess their response to TLR activation or TLR agonist removal. Luminex-based assays and enzyme-linked immunosorbent assays were used to measure cytokine/chemokine and immunoglobulin levels in serum and cytokine levels in cell culture studies. In vitro cell culture was used to assess macrophage response to cell death stimuli, TLR activation, and M1/M2 polarization. Data were compared using the Mann–Whitney
U
test.
Results
Loss of caspase-8 expression in macrophages promotes onset of a mild systemic inflammatory disease, which is preventable by the deletion of RIPK3. In vitro cell culture studies reveal that caspase-8–deficient macrophages are prone to a caspase-independent death in response to death receptor ligation; yet, caspase-8–deficient macrophages are not predisposed to unchecked survival, as analysis of mixed bone marrow chimeric mice demonstrates that caspase-8 deficiency does not confer preferential expansion of myeloid populations. Loss of caspase-8 in macrophages dictates the response to TLR activation, as injection of TLR ligands upregulates expression of costimulatory CD86 on the Ly6C
high
CD11b
+
F4/80
+
splenic cells, and oral antibiotic treatment to remove microbiota prevents splenomegaly and lymphadenopathy in
Cre
LysM
Casp8
fl/fl
mice. Further, caspase-8–deficient macrophages are hyperresponsive to TLR activation and exhibit aberrant M1 macrophage polarization due to RIPK activity.
Conclusions
These data demonstrate that caspase-8 functions uniquely in macrophages by controlling the response to TLR activation and macrophage polarization in an RIPK-dependent manner.
Publisher
BioMed Central,BioMed Central Ltd,Springer Nature B.V
Subject
/ Animals
/ Antigens, Differentiation - immunology
/ Antigens, Differentiation - metabolism
/ Enzymes
/ Female
/ Macrophage Activation - immunology
/ Medicine
/ Receptor-Interacting Protein Serine-Threonine Kinases - genetics
/ Receptor-Interacting Protein Serine-Threonine Kinases - immunology
/ Receptor-Interacting Protein Serine-Threonine Kinases - metabolism
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