Introduction

Every chemical compound absorbs, transmits, or reflects light (electromagnetic radiation) over a certain
range of wavelength. Spectrophotometry is a measurement of how much a chemical substance absorbs
or transmits. Spectrophotometry is widely used for quantitative analysis in various areas (e.g.,
chemistry, physics, biology, biochemistry, material and chemical engineering, clinical applications,
industrial applications, etc). Any application that deals with chemical substances or materials can use
this technique. In biochemistry, for example, it is used to determine enzyme-catalyzed reactions. In
clinical applications, it is used to examine blood or tissues for clinical diagnosis. There are also several
variations of the spectrophotometry such as atomic absorption spectrophotometry and atomic emission
spectrophotometry.

A spectrophotometer is an instrument that measures the amount of photons (the intensity of light)
absorbed after it passes through sample solution. With the spectrophotometer, the amount of a known
chemical substance (concentrations) can also be determined by measuring the intensity of light
detected. Depending on the range of wavelength of light source, it can be classified into two different
types:

UV-visible spectrophotometer: uses light over the ultraviolet range (185 - 400 nm) and visible range (400
- 700 nm) of electromagnetic radiation spectrum.

IR spectrophotometer: uses light over the infrared range (700 - 15000 nm) of electromagnetic radiation
spectrum.

In visible spectrophotometry, the absorption or the transmission of a certain substance can be

determined by the observed color. For instance, a solution sample that absorbs light over all visible
ranges (i.e., transmits none of visible wavelengths) appears black in theory. On the other hand, if all
visible wavelengths are transmitted (i.e., absorbs nothing), the solution sample appears white. If a
solution sample absorbs red light (~700 nm), it appears green because green is the complementary color
of red. Visible spectrophotometers, in practice, use a prism to narrow down a certain range of
wavelength (to filter out other wavelengths) so that the particular beam of light is passed through a
solution sample.

Devices and mechanism

Figure 1 illustrates the basic structure of spectrophotometers. It consists of a light source, a collimator, a
monochromator, a wavelength selector, a cuvette for sample solution, a photoelectric detector, and a
digital display or a meter. Detailed mechanism is described below. Figure 2 shows a sample
spectrophotometer (Model: Spectronic 20D).
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Figure 1: Basic structure of spectrophotometers (CC BY-4.0; Heesung Shim via LibreTexts)

A spectrophotometer, in general, consists of two devices; a spectrometer and a photometer. A

spectrometer is a device that produces, typically disperses and measures light. A photometer indicates
the photoelectric detector that measures the intensity of light.

Spectrometer: It produces a desired range of wavelength of light. First a collimator (lens) transmits a
straight beam of light (photons) that passes through a monochromator (prism) to split it into several
component wavelengths (spectrum). Then a wavelength selector (slit) transmits only the desired
wavelengths, as shown in Figure 1.

Photometer: After the desired range of wavelength of light passes through the solution of a sample in
cuvette, the photometer detects the amount of photons that is absorbed and then sends a signal to a
galvanometer or a digital display, as illustrated in Figure 1