Source: Laboratory of Dr. Paul Bower - Purdue University
The method of standard additions is a quantitative analysis method, which is often used when the sample of interest has multiple components that result in matrix effects, where the additional components may either reduce or enhance the analyte absorbance signal. That results in significant errors in the analysis results.
Standard additions are commonly used to eliminate matrix effects from a measurement, since it is assumed that the matrix affects all of the solutions equally. Additionally, it is used to correct for the chemical phase separations performed in the extraction process.
The method is performed by reading the experimental (in this case fluorescent) intensity of the unknown solution and then by measuring the intensity of the unknown with varying amounts of known standard added. The data are plotted as fluorescence intensity vs. the amount of the standard added (the unknown itself, with no standard added, is plotted ON the y-axis). The least squares line intersects the x-axis at the negative of the concentration of the unknown, as shown in Figure 1.
Figure 1. Graphic representation of method of standard addition.
In this experiment, the method of standard additions is demonstrated as an analytical tool. The method is a procedure for the quantitative analysis of a species without the generation of a typical calibration curve. Standard addition analysis is accomplished by measuring spectroscopic intensity before and after the addition of precise aliquots of a known standard solution of the analyte.
This experiment studies non-fluorescent species by reacting them in such a way as to form a fluorescent complex. This approach is commonly used in the investigation of metal ions. Aluminum ions (Al3+) will be determined by forming a complex with 8-hydroxyquinoline (8HQ). The Al3+ is precipitated by 8HQ from aqueous solution and then is extracted into chloroform; the fluorescence of the chloroform solution is measured and related to the concentration of the original Al3+ solution. Sensitivity in the part-per-million (ppm or μg/mL) range is expected for this experiment.
The reaction is
The amount of aluminum in each sample during this experiment is calculated as follows:
Blank | 0 | ||
Unknown + 0 mL Standard | VUnknown(CUnknown) = 25 mL(CUnknown) | ||
Unknown + 1 mL Standard | VUnknown(CUnknown) + VStandard(CStandard) = 25 mL(CUnknown) + 1 mL(1 μg/mL) | ||
Unknown + 2 mL Standard | VUnknown(CUnknown) + VStandard(CStandard) = 25 mL(CUnknown) + 2 mL(1 μg/mL) | ||
Unknown + 3 mL Standard | VUnknown(CUnknown) + VStandard(CStandard) = 25 mL(CUnknown) + 3 mL(1 μg/mL) | ||
Unknown + 4 mL Standard | VUnknown(CUnknown) + VStandard(CStandard) = 25 mL(CUnknown) + 4 mL(1 μg/mL) |
1. Preparing the Reagents
2. Preparing the Samples
3. Selecting the Excitation Wavelength
Determine the excitation and emission wavelengths by running scans, then simply read and record the fluorescence intensity of all samples at those values. The excitation and emission bandwidths are preset at 5 nm. The complex absorbs in the near UV, so the excitation wavelength should be about 385 nm. Initially, monitor the fluorescence at 500 nm in the emission branch.
4. Selecting the Emission Wavelength
Figure 2. Determining optimum EXλmax and EMλmax Wavelengths.
5. Measuring the Fluorescence of the Samples
6. Creating the Standard Addition Plot
A scan of the excitation wavelength from 335–435 showed the highest absorption at 399 nm, so the excitation monochromator was set for that value. Then the emission scan was performed from 450–550 nm, and the strongest signal was found to be at 520 nm. These are the wavelengths that are used for all of the samples.
Sample | Fluorescence Intensity | Corrected Fluorescence Intensity |
Blank | 0.008 | 0.000 |
Sample | 0.128 | 0.120 |
Sample + 1 mL | 0.167 | 0.159 |
Sample + 2 mL | 0.220 | 0.212 |
Sample + 3 mL | 0.260 | 0.252 |
Sample + 4 mL | 0.290 | 0.282 |
A plot of fluorescence (Figure 3) vs. µg of Al3+ added (Figure 4) yielded a least-squares line of:
Fluorescence Intensity = 0.0417 x (µg of Al3+ added) + 0.1216
Amount of Al3+ = -(Y-Int)/Slope = -0.1216/0.0417 = -2.916 µg/mL
Since the amount of unknown added was 25 mL, then the 2.916 µg/mL value needs to be divided by 25.
Unknown Aluminum Concentration = 2.916 µg/mL / 25.0 mL = 0.117 µg/mL = 0.117 ppm
which is quite close to the actual value of 0.110 ppm (6.4% error).
Figure 3. Fluorescence of the samples.
Figure 4. The standard addition calibration plot.
The method of standard additions is often the technique utilized when accurate quantitative results are desired, used in analytical analysis such as atomic absorption, fluorescence spectroscopy, ICP-OES, and gas chromatography. This is often used when there are other components in the sample of interest that causes either a reduction or enhancement of the absorbance desired for quantitative results. When this is the case, one cannot simply compare the analytes signal to standards using the traditional calibration curve approach. In fact, matrix effect evaluation should be a mandatory part of the validation procedure.
Another example where standard additions can be used is when extracting silver from old photographic waste. The waste contains silver halides, and can be extracted so the silver can be reclaimed. By spiking the unknown "waste" with known amounts of silver, this method can predict the amount of silver obtained from the photographic film.
Workers who are exposed to benzene manufacturing plants are often tested to verify they are safely below the accepted levels of benzene. Their urine is tested for the chemical, and that is the biological matrix. Also, the amount of analyte suppression varies for different people, so a single calibration kit will not work. With the method of standard addition, every employee can be tested and evaluated accurately.
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