Introduction to Spectrophotometry PDF

Summary

This document provides an introduction to spectrophotometry, a technique used to measure chemical concentrations using light. It explores the principles behind spectrophotometry and its applications. The document discusses the electromagnetic spectrum, absorption of light, and the Beer-Lambert Law. It describes UV-Vis spectroscopy, explaining the UV-Vis spectrophotometer. The text includes sample problems. It provides a great foundation for understanding spectrophotometry, specifically in chemistry.

Full Transcript

College of Science

Introduction to
Spectrophotometry

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UV-Vis Spectroscopy
UV-Vis spectroscopy is an analytical technique that
measures the amount of discrete wavelengths of UV or visible
light that are absorbed by or transmitted through a sample in
comparison to a reference or blank sample.

Applications:
1. DNA & RNA analysis
2. Pharmaceutical analysis
3. Bacterial culture
4. Beverage analysis
UV-Vis Spectrophotometer
5. Quality assurance

Have been in general use for the last 80 years and over this
period have become the most
important analytical instrument in the modern day laboratory.
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UV-Vis Spectrophotometer

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Cuvettes (Glass or Quartz)

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Spectrophotometry
Spectrophotometry is any technique that uses light to measure
chemical concentrations. Light is both a particle and a wave. Light
waves consist of perpendicular, oscillating electric and magnetic
fields.

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Spectrophotometry
λ Wavelength

ν Frequency is the number of complete oscillations
that the wave makes each second.
The unit of frequency is 1/second.

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Electromagnetic Spectrum
Electromagnetic
spectrum showing
representative molecular
processes that occur
when light in each region
is absorbed. The visible
spectrum spans the
wavelength range 380 to
780 nanometers
(1 nm = 10-9 m).

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Electromagnetic Spectrum
The part of a molecule responsible
for light absorption is called a
chromophore. Any substance
that absorbs visible light appears
colored when white light is
transmitted through it or reflected
from it.

The substance absorbs certain
wavelengths of the white light, and
our eyes detect the wavelengths
that are not absorbed. The
observed color is called the
complement of the absorbed
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Absorption of Light
Absorption of light increases the
energy of a molecule.
Emission of light decreases its
energy.

Visible and ultraviolet radiation promote electrons to higher
energy orbitals.

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Absorption of Light
Sample problem:
By how many kilojoules per mole is the energy of O2 increased when it absorbs
ultraviolet radiation with a wavelength of 147 nm? 1 m = 1x109 nm

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How UV-Vis Spectrophotometer works

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How UV-Vis Spectrophotometer works
Monochromatic light
consists of “one color”
(one wavelength). The
better the
monochromator, the
narrower is the range of Irradiance (I0 or P0)
wavelengths in the or Intensity
emerging beam.
When light is
absorbed by a
sample, the
irradiance of the
beam of light is
decreased.
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How UV-Vis Spectrophotometer works

Transmittance, T, is defined as the fraction of the original light that
passes through the sample.

Beer-Lambert’s Law c = concentration of the sample (M)
(Absorbance) b = pathlength (cm)
ε = molar absorptivity (M-1 cm-1)

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Absorbance, Transmittance, Beer’s Law
Sample problem:
Find the absorbance and transmittance of a 0.00240 M solution of a substance
with a molar absorptivity of 313 M-1 cm-1 in a cell with a 2.00-cm pathlength.

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Limitations to Beer’s Law
Results in non-linear calibration curve.
Affected by high concentration of electrolytes/analyte.
Only true for dilute solution ( 0.01 M).
Scattering of light due to particulates in the sample.
Stray light. Compartments must be tightly closed to
avoid stray light, which leads to false readings.
If too little light gets through the sample (high
absorbance), intensity is hard to measure. If too much
Dilute solutions that are dark colored. light gets through (low absorbance), it is hard to
distinguish transmittance of the sample from that of the
reference.
It is desirable to adjust sample concentration so that
absorbance falls in the intermediate range.

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Standard Calibration Curve
Calibration is the empirical determination of the relationship between a measured quantity and a
known reference or standard value. It is used to establish analytical signal versus concentration
relationships in a calibration or working curve.

A calibration curve shows the response of an
analytical method to known quantities of analyte.

Solutions containing known
concentrations of analyte are called
standard solutions.
Solutions containing all reagents and
solvents used in the analysis, but no
deliberately added analyte, are called
blank solutions. Blanks measure the
response of the analytical procedure to
impurities or interfering species in the
reagents.
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Reference
Harris, D. (2016) Quantitative Chemical Analysis, 9th edition. New York: W.H. Freeman and
Company.

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