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Measurement of optical signal All spectrochemical techniques that operate in the Uvvisible and IR regions of the spectrum employ similar instrumental components 1 The major instrumental differences between emission, photoluminescence, and absorption techniques occur in the arrangement and type of sample introduction system, encoding system and information selection system. All techniques depend upon the measurement of radiant power. The radiant power monitor or optical transducer-signal processing- readout system is shown in block diagram form in Figure 2-9. The specific transducers and signal processing devices used in various regions of the spectrum in specific spectrochemical techniques. In this section we explore how the analytical signal is extracted from the readout data in spectrochemical methods. 2 3 Analytical Signal The analytical signal for emission and chemiluminescence techniques is defined as the signal to be displayed by the readout device due only to analyte emission (EE, it is assumed that EE , is directly related to the radiant power of emission ΦE. ). Similarly, the analytical signal in photoluminescence techniques, EL, is the measured signal due only to radiationally produced emission of the analyte. In the case of absorption methods, the analytical signal is the absorbance A due only to absorption of radiation by the analyte species. 4 Because of the presence of extraneous signals, such as signals from concomitants, the sample cell, and room light, at least two measurements are required to obtain the analytical signal. sources of the background or extraneous signal that registers on the readout device: 1) dark signal Ed of the radiant power monitor: the signal present when no radiation is impingent on the transducer. 2) the background signal, EB due to background radiation that strikes the transducer. The background radiation is composed of radiation from all sources other than the desired optical phenomenon from the analyte. 5 The data domains of the different signals in a spectrochemical instrument prior to the signal processing system are dependent on the observation point. the data are present as an optical radiant power in watts. The transducer can convert this optical signal to an electrical current, voltage, or charge. Normally, the output of the signal processing system to be displayed on the readout device is an electrical voltage. Hence, in general in this book, analyte and background signals will be written as voltages E. 6 Emission and Chemiluminescence Spectrometry The basic instrumental configuration for wavelength resolved emission spectrochemical methods is shown in Figure 2-10. FIGURE 2-10 Instrumentation for emission spectrochemical methods. The excitation source provides the external energy necessary to excite the analyte species. For example, the excitation source could be a flame, a plasma, a high-voltage spark discharge, or a chemical reaction. The sample container holds the sample. The wavelength selector passes a selected wavelength band emitted by the sample to the radiant power monitor 7 The emission that results from excitation of the analyte species by a flame, a plasma, or a chemical reaction encodes the concentration of the analyte as the radiant power of emission ɸE In some spectrochemical methods the excitation source and sample container are an integral unit, as in the nebulizer-burner used in flame emission and the reaction cell used in chemiluminescence. 8 When the analytical sample is present in the same cell, a total or composite signal EtE, is obtained. This total signal is the sum of : EE: Analytical signal Ed: Dark signal EbE: The background emission signal To extract the analytical signal, a second measurement is required to obtain the sum of the dark signal and the background emission signal. This second measurement usually made by replacing the analytical sample with blank that is ideally identical to the analytical sample except that the analyte is missing. 9 If desired, the dark signal can be obtained separately by locking all radiation from reaching the radiant power monitor. The background emission signal could then be obtained from Ebk- Ed. In many instruments the blank solution is used to adjust the readout device to read zero by suppression of the blank signal. This establishment of the zero position is still, however, a measurement of the blank signal. 10 Photoluminescence Spectrometry 11 Here an external source electromagnetic radiation excites the analyte (photoexcitation). The analyte concentration is optically encoded as the luminescent radiant power ɸL , which is measured with the radiant power monitor. The emission wavelength selector that views the luminescence of the sample is typically placed to collect radiation at 90◦ with respect to the excitation axis. Other geometries, such as front surface and 180o, are used in special situations. In some cases only one of the wavelength selectors is necessary. 12 When the analytical sample is placed in the sample ELt: Total luminescence signal EL: analyte luminescence signal, EE: analyte thermal emission signal Ebk Blank signal Ed: dark signal EbE: background emission signal Esc: Scattering signal EbL: Background luminescence signal Analyte and background emission in the UV-visible region are usually significant only in atomic spectroscopy 13 The analyte luminescence signal EL can be obtained with two measurements only if the analyte emission signal EE is small compared to EL, which is often the case. If EE is significant, subtraction of the blank signal gives a measured analyte luminescence signal EL that differs from EL as shown in the equation 14 How EL can be obtained when EE is significant? the excitation source must be turned off. Then the two measurements are made to obtaine EE according to : Subtraction of EE from E’L gives the true analyte luminescence signal. In some cases it is possible to eliminate the measured contribution from analyte emission optically or electronically. For example, if the excitation source is modulated and alternatingcurrent (ac) amplification is used, the ac luminescence signal can be distinguished from the dc emission signal. Often the blank measurement is used to set the zero position of the readout device. 15 Absorption spectrometry FIGURE 2-12 Absorption spectrometer. A narrow spectral band from the radiation source is passed through the sample. The transmitted radiant power is measured by the radiant power monitor. Replacement of the analytical sample by a reference provides a measure of the reference radiant power. The ratio of the radiant power transmitted by the sample to that transmitted by the reference is used to calculate the absorbance A of the sample. 16 The absorption spectrometer is essentially identical to the luminescence spectrometer except that the source, sample cell, and transducer are all on the same optical axis. This permits the measurement of the transmitted radiant power. The shutter allows the user to block the radiation source in order to obtain the dark signal. Usually, only one wavelength selector is required. Absorption measurements can be made in two ways: 1. Transmittance readout 2. Direct absorbance readout Both of these readout schemes are used, although direct absorbance readout is becoming the more common. 17 Transmittance readout The ideal or true transmittance T is the ratio of radiant power passed by the analyte to the radiant power passed by an ideal blank. It could be obtained by: (1) measuring the signal Es that results from the source radiant power passing through the analytical sample, (2) measuring the signal Er, that results from the source radiant power passing through the ideal blank or reference solution; and (3) obtaining the transmittance as in 18 In practice, however, the presence of other signals (dark signal, background emission) necessitates a third measurement. The measured transmittance T' is defined by the equation Est: total sample signal obtained with the source shutter open and the analytical sample in the sample container E0t is the zero percent transmittance (0% T) signal obtained with the shutter closed and the blank in the sample container, Ert is the 100% transmittance (100% T) signal obtained with the shutter open and the blank (reference) in the sample container. 19 The 0% T signal E0t is composed of any background emission EbE and dark current Ed as shown by the equation When the blank is in the sample container and the shutter open, the measured total reference signal Ert called the 100% T signal, is composed of : the reference transmission signal Er the 0% T signal and any background luminescence EbL 20 When the analytical sample is in the sample container and the shutter is open, the measured signal is Est, the total sample signal. This signal is given by where Es is the sample transmission signal, EE is the analyte emission signal, and EL is the analyte luminescence signal. Er>>EbL T‘= T only when ES>>EL+EE+EbL 21 If one or more of the signals EL, EE, or EbL, is significant, several additional measurements must be made to correct equation 2-31 to obtain the true transmittance, information selection techniques criminate against the extraneous or additional must be used signals. As in a photoluminescence techniques, analyte and background emission are usually significant only for atomic spectrometry. The measured transmittance T' is then used to calculate an absorbance A' = -log T' which is an approximation to the true absorbance A = -log T. 22 Direct Absorbance Readout As part of the signal processing electronics, many modern absorption spectrometers have provision for obtaining and displaying absorbance directly. The true absorbance A is given by where EA is the voltage proportional to the analyte absorbance and k' is a logarithmic conversion factor in volts per absorbance unit. The voltage EA and hence A are found from two measurements: 1. a reference logarithmic voltage or zero absorbance Elr, is obtained with the shutter open and the blank in the sample container; 2. Then a sample logarithmic voltage Els is obtained with the shutter open and the analytical sample in the sample container 23 The voltage EA is then given by The voltages Els, and Elr, are logarithmically related to Es and Er, as follows: a constant reference voltage Often Elris set to zero on the readout device so that Els, is read out directly as EA. 24 Note that in the two-step absorbance measurement scheme, a measurement is not made with the light source shutter closed (0% T) since A would be infinity. Thus (Ed + EbE) must be negligible compared to Es and Er or electronically or optically set to zero by other means. Also, EE + EbL + EL must be negligible so that Es = Est and Er = Ert otherwise, the measured absorbance A' only approximates the true absorbance A. 25 26 Modulators Several types of devices are used to amplitude modulate a radiation source (see Section 4-5). Modulation is based on mechanical interruption of a light beam or on electro-optic, magneto-optic, or acousto-optic phenomena. Mechanical Choppers Mechlanical modulators or choppers provide a controlled periodic physical blocking of a radiation beam. The lnost common mechanical modulators are based on a rotating disk or wheel with apertures or vanes as shown in Figure 3-14a and b. 27 28 The chopping frequency is determined by the number of apertures and the rotation rate of the shaft of the motor. The maximum modulation frequency is generally in the range 1 to 10kHz. Vibrating or tuning fork modulators are based on periodic lateral movement of one or two vanes in and out of the light path as illustrated in Figure 3-14c. Because these are resonant devices, a given chopper is designed to operate at one frequency (10 to 6000 Hz). The modulation waveform depends on the size, shape, and configuration of the vanes and can be sinusoidal. 29 Other types of resonant choppers include oscillating choppers based on torsion rod and taut band designs (Figure 3-14d), which rely on rotation of a vane in and our of the light path. Choppers can be used for specialized functions by ounting mirrors, refractor plates, gratings, or filters to the vanes. 30 Electro-optic and magneto-optic modulators 31 32