Bio-Protocol (Jan 2016)

Super-resolution Imaging of Live BY2 Cells Using 3D-structured Illumination Microscopy

  • Karen Bell,
  • Karl Oparka,
  • Kirsten Knox

DOI
https://doi.org/10.21769/BioProtoc.1697
Journal volume & issue
Vol. 6, no. 1

Abstract

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Light microscopy is the standard tool for studying sub-cellular structures however, owing to the diffractive properties of light, resolution is limited to 200 nm. Super-resolution microscopy methods circumvent this limit, offering greater resolution, particularly when studying fluorescently labeled sub-cellular structures. Super-resolution methods such as 3D-SIM (Structured Illumination Microscopy) fill a useful niche between confocal and electron microscopy. We have previously had success using fixed plant tissue samples with 3D-SIM (Bell and Oparka, 2014). However, sensitive structures can be altered by fixation and embedding procedures, so we developed a method for imaging live cells. In this protocol we used 3D-SIM to image the ER and Hechtian Strands in live, plasmolysed BY2 cells.