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Also known as: capillary analysis

Gas chromatographic detectors sense the solute vapours in the mobile phase as they emerge from the column. Thermal-conductivity detectors compare the heat-conducting ability of the exit gas stream to that of a reference stream of pure carrier gas. To accomplish this, the gas streams are passed over heated filaments in thermal-conductivity cells. Measured changes in filament resistance of the cells reflect temperature changes caused by increments in thermal conductivity. This resistance change is monitored and registered continuously on a recorder. An alternate type of detector is the flame-ionization detector, in which the gas stream is mixed with hydrogen and burned. Positive ions and electrons are produced in the flame when organic substances are present. The ions are collected at electrodes and produce a small, measurable current. The flame-ionization detector is highly sensitive to hydrocarbons, but it will not detect carrier gases, such as nitrogen, or highly oxidized materials, such as carbon dioxide, carbon monoxide, sulfur dioxide, and water. In another device, the electron-capture detector, a stream of electrons from a radioactive source is produced in a potential field. Materials in the gas stream containing atoms of certain types capture electrons from the stream and measurably reduce the current. The most important of the capturing atoms are the halogensfluorine, chlorine, bromine, and iodine. This type of detector, therefore, is particularly useful with chlorinated pesticides. Certain elements will emit light of distinctive wavelength when excited in a flame. The flame photometric detector measures the intensity of light with a photometric circuit. Solute species containing halogens, sulfur, or phosphorus can be burned to produce ionic species containing these elements and the ions sensed by electrochemical means.

Liquid chromatographic detectors

Liquid chromatographic detectors suitable for high-performance columns require clever technology. If the solutes contain structural features that absorb light at certain wavelengths, the decrease in the intensity of the transmitted beam of light compared to the intensity of the incident beam can be used to monitor the effluent stream. In order for the solute to be detected, it must contain light-absorbing groups, the excitation source must contain light of a wavelength peculiar to this group, and the photoelectric sensor must respond to this wavelength. Also, the mobile phase must be transparent at this wavelength. The scope of solute species detected can be enlarged by reacting a light-insensitive solute with a reagent that contains a light-sensitive group and passing the product through the detector. Solutes may contain groups that absorb light at one wavelength and reemit light of a different wavelength. The fluorescence detector responds to these substances. Light bends or refracts on passing through an interface between air and a liquid or liquid solution. The degree of refraction depends on the nature of the liquid or the composition of the solution. The refractive index detector compares the refraction of the pure mobile phase with that of the column effluent.

Chromatography–mass spectrometry methods

The mass spectrometer is an analytical instrument that bombards molecules with a stream of electrons in a chamber at extremely low pressure to produce a stream of charged fragments that differ in mass. The population of the fragments and the ratio of mass to charge is characteristic of the target molecule. Each fragment is deflected differently in a magnetic field to produce a pattern, the mass spectrum, which can be used to identify the target. The system is a very specific identifying detector when coupled with chromatography. The spectrum can be stored in a computer and compared with entries in a mass spectrum library. For some time the problem with gaseous effluents had been to match the column effluent at one atmosphere pressure to the high-vacuum inlet of the mass spectrometer, while the problem with liquid chromatography had been the large amount of mobile phase entering the ionization chamber of the spectrometer. These incompatibility problems have finally been overcome, and the mass spectrometer is now used in both gas and liquid chromatography. The technology of mass spectrometry is as great, if not greater, than that of chromatography.

If mass spectral data are lacking, solutes in a sample are identified by comparing their behaviour with that of known compounds. In gas chromatography this is best done by determining the retention index of the unknown solute and comparing it with the tabulated data for known compounds on the stationary phase used. Methods exist for estimating the effect of temperature and temperature programming on the retention index.

The area enclosed by a peak, suitably adjusted for the detector response factor for that solute, is proportional to the amount of solute producing the peak. The area is frequently approximated from the peak width and height. Modern electronic integrators will, when properly instructed, ignore electronic noise, compensate for baseline drift, start integration when a peak appears, integrate, and stop the process when the peak exits the detector. Integration, a process of summation, is accomplished by opening and closing a narrow electronic window, registering the signal intensity, repeating the process, and then summing the stored signals to produce a number proportional to the area. The integrator will also sense the peak maximum. The chromatogram is a printed tape with the retention times and peak areas. Programs exist that will incorporate the response factor and calculate the relative peak areas, which give the percentage composition of the sample. Stored mass spectral data may be manipulated to produce the same data. Peak heights are used as quantitative measures for narrow peaks for which the area is difficult to determine accurately.