Mass spectrometer, components

Mass Spectrometry Mass spectrometer components, types of mass spectrometers, ionization sources, and scan types are described in Section 1.1.1. 

TABLE 2.1 Mass Spectrometer Components and Their Functions. 36... 

More recently, a novel technique for the handling of high-matrix samples has been developed that introduces a make-up gas between the spray chamber and the torch. This technique, which has been termed aerosol dilution, does not require the introduction of more water into the system and protects the mass spectrometer components from the high levels of matrix components in the sample. This approach enables the ICP-MS system to directly aspirate 2-3% TDS, with the added benefit... 

The chromatogram can finally be used as the series of bands or zones of components or the components can be eluted successively and then detected by various means (e.g. thermal conductivity, flame ionization, electron capture detectors, or the bands can be examined chemically). If the detection is non-destructive, preparative scale chromatography can separate measurable and useful quantities of components. The final detection stage can be coupled to a mass spectrometer (GCMS) and to a computer for final identification. 

Gas chromatography is not an identification method the components must be identified after their separation by capillary column. This is done by coupling to the column a mass spectrometer by which the components can be identified with the aid of spectra libraries. However tbe analysis takes a long time (a gasoline contains aboutTwo hundred components) so it is not practical to repeat it regularly. Furthermore, analysts have developed te hpiques for identifying... 

Figure Bl.7.4. Schematic diagram of a reverse geometry (BE) magnetic sector mass spectrometer ion source (1) focusing lens (2) magnetic sector (3) field-free region (4) beam resolving slits (5) electrostatic sector (6) electron multiplier detector (7). Second field-free region components collision cells (8) and beam deflection electrodes (9).

Although GGMS is the most widely used ana lytical method that combines a chromatographic sep aration with the identification power of mass spectrometry it is not the only one Chemists have coupled mass spectrometers to most of the mstru ments that are used to separate mixtures Perhaps the ultimate is mass spectrometry/mass spectrome try (MS/MS) m which one mass spectrometer gener ates and separates the molecular ions of the components of a mixture and a second mass spec trometer examines their fragmentation patterns ... 

For mixture.s the picture is different. Unless the mixture is to be examined by MS/MS methods, usually it will be necessary to separate it into its individual components. This separation is most often done by gas or liquid chromatography. In the latter, small quantities of emerging mixture components dissolved in elution solvent would be laborious to deal with if each component had to be first isolated by evaporation of solvent before its introduction into the mass spectrometer. In such circumstances, the direct introduction, removal of solvent, and ionization provided by electrospray is a boon and puts LC/MS on a level with GC/MS for mixture analysis. Further, GC is normally concerned with volatile, relatively low-molecular-weight compounds and is of little or no use for the many polar, water soluble, high-molecular-mass substances such as the peptides, proteins, carbohydrates, nucleotides, and similar substances found in biological systems. LC/MS with an electrospray interface is frequently used in biochemical research and medical analysis. 

Although simple solutions can be examined by these techniques, for a single substance dissolved in a solvent, straightforward evaporation of the solvent outside the mass spectrometer with separate insertion of the sample is usually sufficient. For mixtures, the picture is quite different. Unless the mixture is to be examined by MS/MS methods, it will be necessary to separate it into its individual components. This separation is most often done by gas or liquid chromatography (GC or LC). 

By passing a continuous flow of solvent (admixed with a matrix material) from an LC column to a target area on the end of a probe tip and then bombarding the target with fast atoms or ions, secondary positive or negative ions are ejected from the surface of the liquid. These ions are then extracted into the analyzer of a mass spectrometer for measurement of a mass spectrum. As mixture components emerge from the LC column, their mass spectra are obtained. 

A second use of arrays arises in the detection of trace components of material introduced into a mass spectrometer. For such very small quantities, it may well be that, by the time a scan has been carried out by a mass spectrometer with a point ion collector, the tiny amount of substance may have disappeared before the scan has been completed. An array collector overcomes this problem. Often, the problem of detecting trace amounts of a substance using a point ion collector is overcome by measuring not the whole mass spectrum but only one characteristic m/z value (single ion monitoring or single ion detection). However, unlike array detection, this single-ion detection method does not provide the whole spectrum, and an identification based on only one m/z value may well be open to misinterpretation and error. 

Mixtures passed through special columns (chromatography) in the gas phase (GC) or liquid phase (LC) can be separated into their individual components and analyzed qualitatively and/or quantitatively. Both GC and LC analyzers can be directly coupled to mass spectrometers, a powerful combination that can simultaneously separate and identify components of mixtures. 

As described above, the mobile phase carrying mixture components along a gas chromatographic column is a gas, usually nitrogen or helium. This gas flows at or near atmospheric pressure at a rate generally about 0,5 to 3.0 ml/min and evenmally flows out of the end of the capillary column into the ion source of the mass spectrometer. The ion sources in GC/MS systems normally operate at about 10 mbar for electron ionization to about 10 mbar for chemical ionization. This large pressure... 

As each mixture component elutes and appears in the ion source, it is normally ionized either by an electron beam (see Chapter 3, Electron Ionization ) or by a reagent gas (see Chapter I, Chemical Ionization ), and the resulting ions are analyzed by the mass spectrometer to give a mass spectmm (Figure 36.4). 

In a GC/MS combination, passage of the separated components (A, B, C, D) successively into the mass spectrometer yields their individual spectra. 

By connecting a gas chromatograph to a suitable mass spectrometer and including a data system, the combined method of GC/MS can be used routinely to separate complex mixtures into theii individual components, identify the components, and estimate their amounts. The technique is widely used. 

It is worth noting that some of these methods are both an inlet system to the mass spectrometer and an ion source at the same time and are not used with conventional ion sources. Thus, with electrospray, the process of removing the liquid phase from the column eluant also produces ions of any emerging mixture components, and these are passed straight to the mass spectrometer analyzer no separate ion source is needed. The particle beam method is different in that the liquid phase is removed, and any residual mixture components are passed into a conventional ion source (often electron ionization). 

As each mixture component elutes, the resulting ions are analyzed by the mass spectrometer to give a mass spectrum (Figure 37.4). 

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