Fluorescence polarization microscopy images both the intensity and orientation of fluorescent dipoles, which plays a vital role in studying the molecular structure and dynamics of bio-complex. However, it is difficult to resolve the dipole assemblies on the subcellular structure and their dynamics in living cells with super-resolution. Here we report polarized structured illumination microscopy (pSIM), which decouples the entangled spatial and angular structured illumination through interpreting the dipoles in spatio-angular hyperspace. We demonstrate its application on a series of biological filamentous systems such as cytoskeleton networks and lambda-DNA, and report the dynamics of short actin sliding through myosin-coated surface. Further, pSIM reveals "side-by-side" organization of the actin ring structure in the membrane-associated periodic skeleton in hippocampal neurons. It also images the dipole dynamics of green fluorescent proteins labeled to the microtubules in live U2OS cells. pSIM can be applied directly to a large variety of commercial or home-built SIM systems.
Comment: 18 pages,5 figures, typos fixed