Scanning electron microscopy preparation and analysis of the cell cortex ultrastructure

Abstract

The cellular cortex is a 200-nm-thick actin network that lies beneath the cell membrane. It is responsible for the mechanical properties of the cell and is involved in many cellular processes, such as cell migration and interactions with the environment. To develop a clear view of the structure of this meshwork, high resolution imaging is essential, such as electron microscopy. This technique requires complex sample preparation that can lead to artifacts like shrinkage or hole formation. We present a preparation method that reduces artifacts significantly. Here, the final drying step that is typically performed by critical point drying is replaced by hexamethyldisilazane drying. We quantitatively investigated sample integrity after both preparation methods, and show that there are significant advantages of hexamethyldisilazane drying compared to critical point drying. Furthermore, automated analysis of a network is classically performed by thresholding-based software programs, which are sensitive to noise and uneven brightness of images. The here presented analysis that we have developed is based on a vectorial node algorithm. It reproduces all kinds of networks sufficiently to allow derivation of quantitative network-specific parameters, such as mesh hole size. We use this analysis to compare the network structure of cells prepared by these two drying methods, and show that hexamethyldisilazane drying leads to fewer artificial mesh holes compared to critical point drying. We thus present here a significantly improved method to quantitatively investigate the actin cortex of cells, and show that hexamethyldisilazane drying leads to more accurate imaging compared to critical point drying.Insight Box The highest resolution for imaging the cellular actin cortex is provided by electron microscopy. Scanning electron microscopy samples require a drying process, usually achieved by critical point drying, which is critical for the sample integrity. We compare the structural defects in the actin cortex of hTert RPE1 cells after critical point drying and a chemical based method, namely hexamethyldisilazane drying. In order to characterize the actin network, we also developed a new vectorial based tracing software. We bring here new tool, both experimental and analytical, which will help to streamline studies of the actin cortex.