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SHOCK-D-18-00340-1.pdf

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NIAID Data Ecosystem2026-03-11 收录
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https://figshare.com/articles/dataset/SHOCK-D-18-00340-1_pdf/7800038
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Background: Neutrophil dysfunction plays an important role in inflammation-induced tissue injury. Previously, we identified protein kinase C-d (PKCd) as a critical controller of neutrophil activation and trafficking but how PKCd is regulated in inflammation has not been delineated. PKCd activity is regulated by tyrosine phosphorylation on multiple sites. Tyrosine155 is a key regulator of apoptosis and gene expression, but its role in proinflammatory signaling is not known. Methods: In-vitro studies – superoxide anion (O2 ) and neutrophil extracellular traps (NETs) were measured in bone marrow neutrophils (BMN) isolated from wild type (WT) and PKCdY155F knock-in mice (PKCd tyrosine 155 ! phenylalanine). Our novel 3D biomimetic microfluidic assay (bMFA) was used to delineate PKCd-mediated regulation of individual steps in neutrophil adhesion and migration using WTand PKCdY155F BMN and mouse lung microvascular endothelial cells (MLMVEC). In-vivo studies – WT and PKCdY155F knock-in mice underwent sham or cecal ligation and puncture surgery and the lungs harvested 24 h post-surgery. Results: In vitro – PKCdY155F BMN had significantly reduced O2 and NETs release compared with WT. WT BMN, but not PKCdY155F BMN, demonstrated significant adhesion and migration across tumor necrosis factor-activated MLMVEC in bMFA. PKCd inhibition significantly reduced WT BMN adhesion and migration under low shear and near bifurcations, but had no effect on PKCdY155F BMN. In vivo – mutation of PKCd tyrosine 155 significantly decreased neutrophil migration into the lungs of septic mice. Conclusions: PKCd tyrosine 155 is a key phosphorylation site controlling proinflammatory signaling and neutrophil–endothelial cell interactions. These studies provide mechanistic insights into PKCd regulation during inflammation.
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2019-03-04
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