Wikipedia: Electron microscope

Electron microscope
From Wikipedia, the free encyclopedia.

The electron microscope can magnify very small details due to the use of electrons rather than light to scatter off material, magnifying at levels up to 500,000 times.

History

The first electron microscope was built in 1931 by Ernst Ruska and Max Knoll. It was greatly developed through the 1950s and has allowed great advances in the natural sciences. The advantage of an electron beam is that it has a much smaller wavelength (see wave-particle duality), which allows a higher resolution - the measure of how close together two things can be before they are seen as one. Light microscopes allow a resolution of about 0.2 micrometres, whereas electron microscopes can have resolutions as low as 0.1 nanometers.

Process

Electron beams from a cathode are focused by magnetic lenses on to the specimen. They are then magnified by a series of magnetic lenses until they hit photographic plate or light sensitive sensors - which transfer the image to a computer screen. The image produced is called an electron micrograph (EM).

Types

The Transmission electron microscope (TEM) produces images by detecting electrons that are transmitted through the sample, while the Scanning electron microscope (SEM) produces images by detecting secondary electrons which are emitted from the surface due to excitation by the primary electron beam.

Generally, the TEM resolution is about an order of magnitude better than the SEM resolution, however, because the SEM image relies on surface processes rather than transmission it is able to image bulk samples and has a much greater depth of view, and so can produce images that are a good representation of the 3D structure of the sample.

Treatment

Samples viewed under an electron microscope have to be treated in many ways:

Fixation - is preserving the sample to make it more realistic. Glutaraldehyde - for hardening - and osmic acid - which stains lipids black - are used.
Dehydration - is the removing of water to be replaced with an embedding medium such as ethanol or propanone.
Embedding - supports the tissue for sectioning in a resin such as araldite.
Sectioning - produces thin slices for mounting. These can be cut on an ultramicrotome with a diamond knife to produce very thin slices.
Staining - uses metals such as lead and uranium to reflect electrons to give contrast between different structures.
Ion Beam Milling - thins samples until they are transparent to electrons by firing ions (typically argon) at the surface from an angle and sputtering material from the surface.

Disadvantages

The samples have to be viewed in vacuums, as air would scatter the electrons. This means that no living material can be studied.
The samples have to be prepared in many ways to give proper detail, which may result in artifacts - objects purely the result of treatment, and this gives the problem of distinguishing artifacts from material, particularly in biological samples.

There are some scientists, such as Dr Harold Hillman, who believe that such artefacts are responsible for all the structures observed in biological samples by electron microscopy, rendering the techniques useless for these materials. However, this view is highly controversial.

Electron microscopes are also very expensive to buy and maintain.

Wikipedia articles containing electron microscope images: