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Three-dimensional localization microscopy in live flowing cells
2020
Zenodo
Capturing the dynamics of live cell populations with nanoscale resolution poses a significant challenge, primarily owing to the speed-resolution trade-off of existing microscopy techniques. Flow cytometry would offer sufficient throughput, but lacks subsample detail. Here we show that imaging flow cytometry, in which the point detectors of flow cytometry are replaced with a camera to record 2D images, is compatible with 3D localization microscopy through point-spread-function engineering, which
doi:10.5281/zenodo.3911512
fatcat:6ersfzpnqvgflbmmb3bb2skx7i