Quantitative analysis of lymphocyte membrane protein redistribution from fluorescence microscopy

被引:0
|
作者
Kasson, PM [1 ]
Huppa, JB [1 ]
Davis, MM [1 ]
Brunger, AT [1 ]
机构
[1] Howard Hughes Med Inst, Biophys Program, Stanford, CA 94305 USA
关键词
D O I
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中图分类号
TP31 [计算机软件];
学科分类号
081202 ; 0835 ;
摘要
The relocalization of plasma membrane proteins is critical for establishing cellular polarity and regulating cell signaling. Three-dimensional fluorescence video microscopy allows the dynamic Visualization of proteins in living cells. We have developed a robust and automated method to employ fluorescence data acquired in this manner for quantitative analysis of membrane protein movements across the cell surface. Our method utilizes level-set-based Surface reconstruction followed by a maximum likelihood Surface registration algorithm for rigid-body alignment of noisy images. A surface-walking technique yields distance maps for the cell Surface, which are then used to measure changes in protein Surface distribution over time. Applying this method to signaling in T lymphocytes, we have used it to monitor receptor movements and have validated these results against previously reported single-particle tracking data.
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页码:2933 / 2936
页数:4
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