A DOUBLE BEAM UV-VISIBLE ABSORPTION SPECTROMETER
This page describes a double beam UV-visible absorption spectrometer
in enough detail to meet the requirements of UK-based chemistry courses
for 16 - 18 year olds. The overall design What you are trying to do If you pass white light through a coloured substance, some of the light gets absorbed. A solution containing hydrated copper(II) ions, for example, looks pale blue because the solution absorbs light from the red end of the spectrum. The remaining wavelengths in the light combine in the eye and brain to give the appearance of cyan (pale blue). Some colourless substances also absorb light - but in the ultra-violet region. Since we can't see UV light, we don't notice this absorption. Different substances absorb different wavelengths of light, and this can be used to help to identify the substance - the presence of particular metal ions, for example, or of particular functional groups in organic compounds. The amount of absorption is also dependent on the concentration of the substance if it is in solution. Measurement of the amount of absorption can be used to find concentrations of very dilute solutions. An absorption spectrometer measures the way that the light absorbed by a compound varies across the UV and visible spectrum. A simple double beam spectrometer We'll start with the full diagram, and then explain exactly what is going on at each stage. | |
IMPORTANT! The colour-coding of the light beams through the spectrometer is NOT to show that some light is red or blue or green. The colours are simply to emphasise the two different paths that light can take through the device. Where the light is shown as a blue line, this is the path that it will always take. Where it is shown red or green, it will go either one way or the other - depending on how it strikes the rotating disc (see below). | |
Explaining what's happening
The light source You need a light source which gives the entire visible spectrum plus the near ultra-violet so that you are covering the range from about 200 nm to about 800 nm. (This extends slightly into the near infra-red as well.) | |
Note: "Near UV" and "near IR" simply means the parts of the UV and IR spectra which are close to the visible spectrum. If you aren't happy about how the various types of electromagnetic radiation relate to each other, follow this link before you go on. Use the BACK button on your browser to return here later. | |
You can't get this range of wavelengths from a single lamp, and so a
combination of two is used - a deuterium lamp for the UV part of the
spectrum, and a tungsten / halogen lamp for the visible part. | |
Note: A deuterium lamp contains deuterium gas under low pressure subjected to a high voltage. It produces a continuous spectrum in the part of the UV spectrum we are interested in. | |
The combined output of these two bulbs is focussed on to a diffraction grating. The diffraction grating and the slit You are probably familiar with the way that a prism splits light into its component colours. A diffraction grating does the same job, but more efficiently. By gradually rotating the diffraction grating, you can allow light from the whole spectrum (a tiny part of the range at a time) through into the rest of the instrument. The rotating discs This is the clever bit! Each disc is made up of a number of different segments. Those in the machine we are describing have three different sections - other designs may have a different number.
These are small rectangular glass or quartz containers. They are often designed so that the light beam travels a distance of 1 cm through the contents. The sample cell contains a solution of the substance you are testing - usually very dilute. The solvent is chosen so that it doesn't absorb any significant amount of light in the wavelength range we are interested in (200 - 800 nm). The reference cell just contains the pure solvent. The detector and computer The detector converts the incoming light into a current. The higher the current, the greater the intensity of the light. For each wavelength of light passing through the spectrometer, the intensity of the light passing through the reference cell is measured. This is usually referred to as Io - that's I for Intensity. The intensity of the light passing through the sample cell is also measured for that wavelength - given the symbol, I. If I is less than Io, then obviously the sample has absorbed some of the light. A simple bit of maths is then done in the computer to convert this into something called the absorbance of the sample - given the symbol, A. For reasons which will become clearer when we do a bit of theory on another page, the relationship between A and the two intensities is given by: An absorbance of 0 at some wavelength means that no light of that particular wavelength has been absorbed. The intensities of the sample and reference beam are both the same, so the ratio Io/I is 1. Log10 of 1 is zero. An absorbance of 1 happens when 90% of the light at that wavelength has been absorbed - which means that the intensity is 10% of what it would otherwise be. In that case, Io/I is 100/I0 (=10) and log10 of 10 is 1. | |
Note: If you don't feel comfortable with logarithms, don't worry about it. Just accept that an absorbance scale often runs from zero to 1, but could go higher than that in extreme cases (in other words where more than 90% of a wavelength of light is absorbed). | |
The chart recorder Chart recorders usually plot absorbance against wavelength. The output might look like this: |
Thursday, 27 June 2013
A DOUBLE BEAM UV-VISIBLE ABSORPTION SPECTROMETER
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