Confocal microscopy is an optical imaging technique used to increase optical resolution and contrast of a micrograph by using point illumination and a spatial pinhole to eliminate out-of-focus light in specimens that are thicker than the focal plane.[1] It enables the reconstruction of three-dimensional structures from the obtained images. This technique has gained popularity in the scientific and industrial communities and typical applications are in life sciences, semiconductor inspection and material science.
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Basic concept
The principle of confocal imaging was patented by Marvin Minsky[2] and aims to overcome some limitations of traditional wide-field fluorescence microscopes. In a conventional (i.e., wide-field) fluorescence microscope, the entire specimen is flooded evenly in light from a light source. All parts of the specimen in the optical path are excited at the same time and the resulting fluorescence is detected by the microscope's photodetector or camera including a large unfocused background part. In contrast, a confocal microscope uses point illumination (see Point Spread Function) and a pinhole in an optically conjugate plane in front of the detector to eliminate out-of-focus signal - the name "confocal" stems from this configuration. As only light produced by fluorescence very close to thefocal plane can be detected the image optical resolution, particularly in the sample depth direction, is much better than that of wide-field microscopes. However, as much of the light from sample fluorescence is blocked at the pinhole, this increased resolution is at the cost of decreased signal intensity so long exposures are often required.
As only one point in the sample is illuminated at a time, 2D or 3D imaging requires scanning over a regular raster (i.e. a rectangular pattern of parallel scanning lines) in the specimen. The achievable thickness of the focal plane is defined mostly by the wavelength of the used light divided by the numerical aperture of the objective lens, but also by the optical properties of the specimen. The thin optical sectioning possible make these types of microscopes particularly good at 3D imaging and surface profiling of samples.
Types
Three types of confocal microscopes are commercially available:
- Confocal laser scanning microscopes
- Spinning-disk (Nipkow disk) confocal microscopes
- Programmable Array Microscopes (PAM)
Each of these classes of confocal microscope have particular advantages and disadvantages, most systems are either optimised for resolution or high recording speed (i.e. video capture). Confocal laser scanning microscopes can have a programmable sampling density while Nipkow and PAM use a fixed sampling density defined by the camera resolution. Imaging frame rates are typically very slow for laser scanning systems (e.g. less than 3 frames/second). Commercial spinning-disk confocal microscopes achieve frame rates of over 50 per second[3] - a desirable feature for dynamic observations such as live cell imaging. So the spinning-disk as well as the programmble array microscopes [4] - can be seen as parallel versions of the confocal scanning principle. Cutting edge development of confocal laser scanning microscopy now allows better than video rate (60 frames/second) imaging by using multiple microelectromechanical systems based scanning mirrors.
Confocal x-ray fluorescence imaging is a newer technique that allows control over depth, in addition to horizontal and vertical aiming, for example, when analyzing buried layers in a painting.[5]
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