Applications of spectrophotometry
What is spectrophotometry?
Spectrophotometry is a method to
measure how much a chemical substance absorbs light by measuring the intensity
of light as a beam of light passes through sample solution. The basic principle
is that each compound absorbs or transmits light over a certain range of
wavelength. This measurement can also be used to measure the amount of a known
chemical substance. Spectrophotometry is one of the most useful methods of
quantitative analysis in various fields such as chemistry, physics, biochemistry,
material and chemical engineering and clinical applications.
Principle
The spectrophotometer technique
is to measure light intensity as a function of wavelength. It does this by
diffracting the light beam into a spectrum of wavelengths, detecting the
intensities with a charge-coupled device, and displaying the results as a graph
on the detector and then on the display device.
1.
In the spectrophotometer, a
prism (or) grating is used to split the incident beam into different
wavelengths.
2.
By suitable mechanisms, waves
of specific wavelengths can be manipulated to fall on the test solution. The
range of the wavelengths of the incident light can be as low as 1 to 2nm.
3.
The spectrophotometer is useful
for measuring the absorption spectrum of a compound, that is, the absorption of
light by a solution at each wavelength.
Applications
of Spectrophotometry
1. Concentration
measurement
– Prepare samples
– Make series of standard solutions of known
concentrations
Set spectrophotometer to the λ of
maximum light absorption
− Measure the absorption of the
unknown, and from the standard plot, read the related concentration
2. Detection of
Impurities
•UV absorption spectroscopy is
one of the best methods for determination of impurities in organic molecules.
Additional peaks can be observed due to impurities in the sample and it can be compared with that of standard raw material.
3. Structure
elucidation of organic compounds.
From the location of peaks and
combination of peaks UV spectroscopy elucidate structure of organic molecules:
· the presence or
absence of unsaturation,
· the
presence of hetero atoms
4. Chemical
kinetics
•Kinetics of reaction can also be
studied using UV spectroscopy. The UV radiation is passed through the reaction
cell and the absorbance changes can be observed.
5. Detection of
Functional Groups
•Absence of a band at particular
wavelength regarded as an evidence for absence of particular group
6. Molecular
weight determination
•Molecular weights of compounds
can be measured spectrophotometrically by preparing the suitable derivatives of
these compounds.
•For example, if we want to determine the molecular weight of amine
then it is converted in to amine picrate.
Test sensitivity and
specificity
• Sensitivity refers to
the lower limit of detection, or the lowest concentration capable of being
detected by a test method.
• Failure to detect small
amounts of a substance in a test will result in a false-negative result.
• Specificity refers to
the ability to detect only the substance for which the test is designed.
• Reaction with other substances (cross-reactivity ) decreases the specificity of the test and can cause false positive results .
Some
General Applications
Ø
Detection
of concentration of substances
Ø
Detection
of impurities
Ø
Structure
elucidation of organic compounds
Ø
Monitoring
dissolved oxygen content in freshwater and marine ecosystems
Ø
Characterization
of proteins
Ø
Detection
of functional groups
Ø
Respiratory
gas analysis in hospitals
Ø
Molecular
weight determination of compounds
Ø
The
visible and UV spectrophotometer may be used to identify classes of compounds
in both the pure state and in biological preparations.
Applications of Spectrophotometry in
biological sciences
Ø The theories and techniques of measuring the
absolute values of the transmittance and reflectance of translucent biological
materials with opal glass plates are presented. These methods were called opal glass transmission and reflection methods. They are simple and easy to
practice with spectro-photometers commonly used for the measurement of
transparent materials. From the transmission and reflection spectra of leaves
observed by these methods, it was proved that they give us the exact values of
the transmittance and reflectance.
Ø From the results of the measurements by opal
glass transmission and reflection methods, it was found that we need to define
at least six quantities, which describe the optical properties of translucent
or non-transparent biological materials.
Ø The way
and use of evaluating these properties are described, especially paying attention
to the absolute measurement of the light absorbed by those samples.
Ø By modifying the opal glass reflection method,
we can observe the logarithm of the reciprocal of the relative value of
reflectance, even more simply than by opal glass reflection method for absolute
measurement. The measurements by the modified method showed clear absorption
bands of biological non-transparent materials. As one of the application of the
method, the state of carotenoids in vivo was
studied. The results indicated that some carotenoids exists in their
crystalline state in roots or fruits.
Spectrophotometry
applications in Analysis of a biochemical mixture
Spectrophotometric
analysis is essential for determining biomolecule concentration of a solution
and is employed ubiquitously in biochemistry and molecular biology.
The application of the Beer‐Lambert‐BouguerLawis
routinely used to determine the concentration of DNA, RNA or protein.
There is however a
significant difference in determining the concentration of a given species
(RNA, DNA, protein) in isolation (a contrived circumstance) as opposed to
determining that concentration in the presence of other species (a more
realistic situation).
To present the student with a more realistic
laboratory experience and also to fill a hole that we believe exists in student
experience prior to reaching a biochemistry course,
We have devised a three week laboratory
experience designed so that students learn to connect laboratory practice with
theory, apply the Beer‐Lambert‐Bougert Law to biochemical analyses,
Demonstrate the utility and limitations of
example quantitative colorimetric assays, demonstrate the utility and
limitations of UV analyses for biomolecules, develop strategies for analysis of
a solution of unknown biomolecular composition,
Use digital
micropipettors to make accurate and precise measurements, and apply graphing
software.
Application in DNA and RNA Concentration
Spectrophotometry can be used to estimate DNA or RNA
concentration and to analyze the purity of the preparation. Typical wavelengths
for measurement are 260 nm and 280 nm. In addition measurements at 230 nm and
320 nm can provide further information. Purines and pyrimidines in nucleic
acids naturally absorb light at 260 nm.
For pure samples it is well documented that for a
pathlength of 10 mm, an absorption of 1A unit is equal to a concentration of 50
µg/ml DNA and 40 µg/ml for RNA. For oligonucleotides the concentration is
around 33 µg/ml but this may vary with length and base sequence. So for DNA:
Concentration (µg/ml) = Abs260 × 50.
These values are known as conversion factors. A
number of other substances which also absorb light at 260 nm could interfere
with DNA values, artificially increasing the result calculated from the
absorption readings. To compensate for this a selection of ratios and
background corrections have been developed to help eliminate false readings.
Wavelength scan for a
pure DNA sample
There is a wide
absorbance peak around 260 nm preceded by a ‘dip’ at 230 nm. Therefore to
measure the DNA absorption, the 260 nm DNA peak must be distinguishable from
the 230 nm reading. If the readings at 230 nm are too similar to those at 260
nm, DNA cannot be measured accurately.
Higher 230 nm readings
can indicate contaminants in the sample. There should also be a rapid tail-off
from 260 nm down to 320 nm. For this reason, 320 nm is often used to measure
background (see background correction).
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