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Mass Spectrometer Characteristics

The mass spectra of atenolol and compound were obtained by direct insertion of the sample into CEC 21-Ho B mass spectrometer. Characteristics of these mass spectra are summarized in Tables 5. and 6, and Pig. 5 The ion source temperature was 15o°C and 2oo-25o°C, respectively, and the ionizing electron beam energy was 7o eV. [Pg.14]

In GC-MS effluent from the column is introduced directly into the mass spectrometer s ionization chamber in a manner that eliminates the majority of the carrier gas. In the ionization chamber all molecules (remaining carrier gas, solvent, and solutes) are ionized, and the ions are separated by their mass-to-charge ratio. Because each solute undergoes a characteristic fragmentation into smaller ions, its mass spectrum of ion intensity as a function of mass-to-charge ratio provides qualitative information that can be used to identify the solute. [Pg.571]

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. [Pg.216]

Atoms of elements are composed of isotopes. The ratio of natural abundance of the isotopes is characteristic of an element and is important in analysis. A mass spectrometer is normally the best general instrument for measuring isotope ratios. [Pg.424]

Effusion separator (or effusion enricher). An interface in which carrier gas is preferentially removed from the gas entering the mass spectrometer by effusive flow (e.g., through a porous tube or through a slit). This flow is usually molecular flow, such that the mean free path is much greater than the largest dimension of a traverse section of the channel. The flow characteristics are determined by collisions of the gas molecules with surfaces flow effects from molecular collisions are insignificant. [Pg.432]

Quantitative mass spectrometry, also used for pharmaceutical appHcations, involves the use of isotopicaHy labeled internal standards for method calibration and the calculation of percent recoveries (9). Maximum sensitivity is obtained when the mass spectrometer is set to monitor only a few ions, which are characteristic of the target compounds to be quantified, a procedure known as the selected ion monitoring mode (sim). When chlorinated species are to be detected, then two ions from the isotopic envelope can be monitored, and confirmation of the target compound can be based not only on the gc retention time and the mass, but on the ratio of the two ion abundances being close to the theoretically expected value. The spectrometer cycles through the ions in the shortest possible time. This avoids compromising the chromatographic resolution of the gc, because even after extraction the sample contains many compounds in addition to the analyte. To increase sensitivity, some methods use sample concentration techniques. [Pg.548]

Mass Spectrometry. As of 1996, ms characteristics of pyrazoles and derivatives had not been described in depth. The fate of unsubstituted pyrazole (23) in the mass spectrometer operated in the electron ionization mode may be depicted as follows ... [Pg.308]

Mass spectrometers exploit the difference in the mass-to-charge (m/z) ratio of ionized atoms or molecules to separate them from each other. The m/z ratio of a molecule is also a highly characteristic property that can be used for determining chemical and structural information. Further, molecules can be fragmented in distinctive ways in mass spectrometers, and the fragments that arise also provide quite specific structural information about the molecule. The basic... [Pg.136]

Aliphatic amines undergo a characteristic a cleavage in the mass spectrometer, similar to that observed for alcohols. A C-C bond nearest the nitrogen atom is broken, yielding an alkyl radical and a resonance-stabilized, nitrogen-containing cation. [Pg.416]

Every mass spectrometer consists of four principal components (Fig 1) (1) the source, where a beam of gaseous ions are produced from the sample (2) the analyzer, where the ion beam is resolved into its characteristic mass species (3) the detector, where the ions are detected and their intensities measured (4) the sample introduction system to vaporize and admit the sample into the ion source. There is a wide variety in each of these components and only those types which are relevant to analytical and organic mass spectrometry will be emphasized in this survey. The instrumentation... [Pg.37]

The power of mass spectrometry lies in the fact that the mass spectra of many compounds are sufficiently specific to allow their identification with a high degree of confidence, if not with complete certainty. If the analyte of interest is encountered as part of a mixture, however, the mass spectrum obtained will contain ions from all of the compounds present and, particularly if the analyte of interest is a minor component of that mixture, identification with any degree of certainty is made much more difficult, if not impossible. The combination of the separation capability of chromatography to allow pure compounds to be introduced into the mass spectrometer with the identification capability of the mass spectrometer is clearly therefore advantageous, particularly as many compounds with similar or identical retention characteristics have quite different mass spectra and can therefore be differentiated. This extra specificity allows quantitation to be carried out which, with chromatography alone, would not be possible. [Pg.21]

An advantage of the mass spectrometer as a detector is that it may allow differentiation of compounds with similar retention characteristics or may allow the identification and/or quantitative determination of components that are only partially resolved chromatographicaUy, or even those that are totally unresolved. This may reduce the time required for method development and is discussed in more detail in Chapter 3. [Pg.35]

The great advantage of the mass spectrometer is its abihty to use mass, more accurately the mass-to-charge ratio, as a discriminating feature. In contrast to, for example, the UV detector, which gives rise to broad signals with little selectivity, the ions in the mass spectrum of a particular analyte are often characteristic of that analyte. Under these conditions, discrete signals, which may be measured accurately and precisely, may be obtained from each analyte when they are only partially resolved or even completely umesolved from the other compounds present. [Pg.38]

A more definitive identification may be obtained by combining retention characteristics with more specific information from an appropriate detector. Arguably, the most information-rich HPLC detectors for the general identification problem are the diode-array UV detector, which allows a complete UV spectrum of an analyte to be obtained as it elutes from a column, and the mass spectrometer. The UV spectrum often allows the class of componnd to be determined but the... [Pg.39]

The most widely used LC detector, and the one which, other than the mass spectrometer, gives the most insight into the identity of an analyte, is probably the UV detector, although a UV spectrum very rarely allows an unequivocal identification to be made. It may allow the class of compound to be identified and this, together with the retention characteristics of the analyte, can provide the analyst with a better indication of the identity of the analyte. In the vast majority of cases, however, identification with complete certainty cannot be achieved. [Pg.50]

The need for a more definitive identification of HPLC eluates than that provided by retention times alone has been discussed previously, as have the incompatibilities between the operating characteristics of liquid chromatography and mass spectrometry. The combination of the two techniques was originally achieved by the physical isolation of fractions as they eluted from an HPLC column, followed by the removal of the mobile phase, usually by evaporation, and transfer of the analyte(s) into the mass spectrometer by using an appropriate probe. [Pg.133]

Selected-ion monitoring A technique in which the mass spectrometer is used to monitor only a small number of ions characteristic of the analyte of interest. [Pg.310]

Another complicating characteristic of materials from the environment is that the size and nature of the residue to be analyzed in the mass spectrometer will change from sample to sample. To determine if this might have an effect on the observed TCDD signal, we analyzed identical samples of TCDD with differing amounts of squalane, a saturated hydrocarbon selected as a model for residues obtained from standard extraction and cleanup procedures. As is indicated in Table I (Part A), there was... [Pg.100]

See other pages where Mass Spectrometer Characteristics is mentioned: [Pg.35]    [Pg.178]    [Pg.35]    [Pg.178]    [Pg.534]    [Pg.568]    [Pg.173]    [Pg.195]    [Pg.277]    [Pg.283]    [Pg.539]    [Pg.41]    [Pg.528]    [Pg.531]    [Pg.615]    [Pg.86]    [Pg.178]    [Pg.178]    [Pg.406]    [Pg.568]    [Pg.253]    [Pg.635]    [Pg.736]    [Pg.18]    [Pg.207]    [Pg.995]    [Pg.367]    [Pg.162]    [Pg.467]    [Pg.207]   


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Characteristic mass

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