The Abbe diffraction limit edit

Observation of sub-wavelength structures with microscopes is difficult because of the Abbe diffraction limit. Ernst Abbe found in 1873 that light with wavelength λ,travelling in a medium with refractive index n and converging to a spot with angle φ will make a spot with radius

${\displaystyle d={\frac {0.61\lambda }{nsin\phi }}}$ 

The denominator nsinφ is called the numerical aperture (NA) and can reach about 1.4 in modern optics, hence the Abbe limit is roughly d=λ/2. With green light around 500nm the Abbe limit is 250nm which is large compared to most nanostructures or biological cells with sizes on the order of 1μm and their internal organelles being much smaller. To increase the resolution, shorter wavelengths can be used such as UV and X-ray microscopes. These techniques offer splendid resolution but are expensive, suffer from lack of contrast in biological samples, and also tend to damage the sample.

Resources edit

• Microscope optics
• Microscopy Primer
• Olympus Interactive Java Tutorials on Microscopy
• Nikon MicroscopyU with interactive tutorials on microscopy techniques

The optical microscope edit

Bright Field edit

The light is sent to the sample in the same directions as you are looking - most things will look bright unless they absorb the light.

Dark Field edit

Light is sent towards the sample at an angle to your viewing direction and you only see light that is scattered. This makes most images appear dark and only edges and curved surfaces will light up.

Polarized Light edit

DIC vs H edit

Confocal laser scanning microscopy is a technique that allows a much better resolution from optical microscopes and three dimensional imaging. A review can be found in Paddock, Biotechniques 1999

Using a high NA objective also gives a very shallow depth of focus and hence the image will be blurred by structures above or below the focus point in a classical microscope. A way to circumvent this problem is the confocal microscope, or even better the Laser Scanning Confocal Microscope (LSCM). Using a laser as the light source gives better control of the illumintaion, especially when using fluorescent markers in the sample. The theoretical resolution using a 1.4 NA objective can reach 140nm laterally and 230nm vertically ^[1] while the resolution quoted in ref ^[2] is 0.5×0.5×1μm. The image in the LSCM is made by scanning the sample in 2D or 3D and recordning the signal for each point in space on a PC which then generates the image.

X-ray microscopy uses X-rays to image with much shorter wavelength than optical light, and hence can provide much higher spatial resolution and use different contrast mechanisms. X-ray microscopy allows the characterization of materials with submicron resolution approaching the 10's of nanometers. X-ray microscopes can use both laboratory x-ray sources and synchrotron radiation from electron accelerators. X-ray microscopes using synchrotron radiation provide the greatest sensitivity and power, but are unfortunately rather large and expensive. X-ray microscopy is usually divided into two overlapping ranges, referred to as soft x-ray microscopy (100eV - 2keV) and hard x-ray microscopy (1keV-40keV). All x-rays penetrate materials, more for higher energy x-rays. Hence, soft x-ray microscopy provides the best contrast for small samples. Hard x-rays do have the ability to pass nearly unhindered through objects like your body, and hence also give rather poor contrast in many of the biological samples you would like to observe with the x-ray microscope. Nevertheless, hard x-ray microscopy allows imaging by phase contrast, or using scanning probe x-ray microscopy, by using detection of fluorescent or scattered x-rays. Despite its limitations, X-ray microscopy is a powerful technique and in some cases can provide characterization of materials or samples that cannot be done by any other means.

vIdentification of the functional groups present in a nanomaterial is a frequent requirement in nanoscience and nanotechnology research. Among other tools, FT-IR has found much popularity among researches due to its versatility, relative ease of use and ability to use as a quantification tool.

Atoms in a chemical bonds constantly vibrate. This vibration can be analogue to a system with two masses attached to a spring. The vibration frequency depend upon the weight of the masses and the spring constant of the connecting spring. In the same way, depending on the masses of the atoms that contributes to a bond and cohesiveness of the bond, frequency differ. Since bonds have atoms with different shapes and sizes and different strength, each combination of atoms in an each type of bond has a unique harmonic frequency. This natural frequency lies in the range of infrared region and therefore a spectroscopic method that use IR can be devised to analyze bond vibrations.

When the IR radiation with the same harmonic frequency of the bond shines upon the bond. The bond vibration is amplified by increased transfer of energy from the IR radiation. When range of IR frequencies given to the material, it only absorb IR frequencies that corresponds to the natural frequencies of the bonds that exist in the sample. Others are not absorbed and can be analyzed using an Infrared spectrometer, which tells you the frequencies that are absorbed by the sample. This provides important information about the functional groups present in the sample. This is exactly what FT-IR does.

As FT-IR can be used to get information about functional groups present in nanomaterials. This is particularly useful in cases such as when one attempts to surface modify nanomaterials to increase affinity, reactivity or compatibility. Analyzing the FT-IR of a nanomaterial would tell you what groups present and then appropriate surface modification strategy be decided based on the groups present. Further, it can also be useful in characterizing the surface modification has taken place, as new groups should emerge if the reaction is successful.Identification of the functional groups present in a nanomaterial is a frequent requirement in nanoscience and nanotechnology research. Among other tools, FT-IR has found much popularity among researches due to its versatility, relative ease of use and ability to use as a quantification tool.

Atoms in a chemical bonds constantly vibrate. This vibration can be analogue to a system with two masses attached to a spring. The vibration frequency depend upon the weight of the masses and the spring constant of the connecting spring. In the same way, depending on the masses of the atoms that contributes to a bond and cohesiveness of the bond, frequency differ. Since bonds have atoms with different shapes and sizes and different strength, each combination of atoms in an each type of bond has a unique harmonic frequency. This natural frequency lies in the range of infrared region and therefore a spectroscopic method that use IR can be devised to analyze bond vibrations.

When the IR radiation with the same harmonic frequency of the bond shines upon the bond. The bond vibration is amplified by increased transfer of energy from the IR radiation. When range of IR frequencies given to the material, it only absorb IR frequencies that corresponds to the natural frequencies of the bonds that exist in the sample. Others are not absorbed and can be analyzed using an Infrared spectrometer, which tells you the frequencies that are absorbed by the sample. This provides important information about the functional groups present in the sample. This is exactly what FT-IR does.

As FT-IR can be used to get information about functional groups present in nanomaterials. This is particularly useful in cases such as when one attempts to surface modify nanomaterials to increase affinity, reactivity or compatibility. Analyzing the FT-IR of a nanomaterial would tell you what groups present and then appropriate surface modification strategy be decided based on the groups present. Further, it can also be useful in characterizing the surface modification has taken place, as new groups should emerge if the reaction is successful.

• Raman scattering
• Resonance Raman spectroscopy

Surface Enhanced Raman Spectroscopy (SERS) edit

• Surface Enhanced Raman Spectroscopy (SERS)
• Surface-enhanced Raman spectroscopy: a brief retrospective

See also notes on editing this book Nanotechnology/About#How_to_contribute.

1. ↑ Confocal laser scanning microscopy, Paddock SW, Biotechniques , vol. 27 (5): 992 NOV 1999
2. ↑ A new UV-visible confocal laser scanning microspectrofluorometer designed for spectral cellular imaging, Favard C, Valisa P, Egret-Charlier M, Sharonov S, Herben C, Manfait M, Da Silva E, Vigny P, Biospectroscopy , vol. 5 (2): 101-115 1999