IL-8-induced L-selectin shedding regulates its binding kinetics to PSGL-1

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JIA XiaoLing CHEN Juan LONG Mian National Microgravity Laboratory Institute of Mechanics Chinese Academy of Sciences Beijing China Center of Biomechanics and Bioengineering Institute of Mechanics Chinese Academy of Sciences Beijing China School of Biological Science and Medical Engineering Beihang University Beijing China [1 ,2 ,3 ,1 ,2 ,1 ,2 ,1 ,100190 ,2 ,100190 ,3 ,100083 ]
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L-selectin plays a crucial role in inflammation cascade by initiating the tethering and rolling of leukocytes on endothelium wall. While many L-selectin molecules are rapidly shed from the cell surface upon activation, the remaining membrane-anchored L-selectin may still play an important role in regulating leukocyte rolling and adhesion with different binding kinetics. Here we developed an in vitro model to activate Jurkat cells via interlukin-8 (IL-8) and quantified the two-dimensional (2D) binding kinetics, using a micropipette aspiration assay, of membrane-anchored L-selectin to P-selectin glycoprotein ligand 1 (PSGL-1) ligand coupled onto human red blood cells (RBCs). The data indicated that L-selectin shedding reduced the amount of membrane-anchored L-selectin and lowered both its reverse and forward rates. These results suggested that the rolling dynamics of activated leukocytes was determined by two opposite impacts: reducing the surface presentation would enhance the rolling but lowering the kinetic rates would decrease the rolling. This finding provides a new insight into under-standing how L-selectin shedding regulates leukocyte rolling and adhesion.
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页码:2786 / 2793
页数:8
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