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High performance liquid chromatography mass spectrometer

High performance liquid chromatography - mass spectrometer... [Pg.400]

A new technique that resembles the GC-MS technique described here is high-performance liquid chromatography-mass spectrometry (HPLC-MS). An HPLC instrument is coupled through a special interface to a mass spectrometer. The substances that elute from the HPLC column are detected by the mass spectrometer, and their mass spectra can be displayed, analyzed, and compared with standard spectra found in the computer library built into the instrument. [Pg.394]

Berger U, Langlois I, Oehme M et al (2004) Comparison of three types of mass spectrometer for high-performance liquid chromatography/mass spectrometry analysis of perfluor-oaUcylated substances and fluorotelomer alcohols. Eur J Mass Spectrom 10 579-588... [Pg.61]

GC = gas chromatography ECD = electron capture detector EIA = enzyme-immunoassay GPC = gel permeation chromatography HPLC = high-performance liquid chromatography ITMS = ion trap mass spectrometer LSE = liquid solid extraction MS = mass spectrometry RSD = relative standard deviation SPE = solid phase extraction... [Pg.259]

Reversed-phase high-performance liquid chromatography (HPLC) column 50 mm x 3.2-mm i.d. with Kromasil 5- um Gig packing High-performance liquid chromatograph coupled to a triple-quadrupole mass spectrometer with an atmospheric pressure chemical ionization (APCI) source Gel permeation chromatograph with a 60 mm x 25-mm i.d. column packed with Bio-Beads SX-3 (50-g)... [Pg.1169]

In addition to GC/MS, high performance liquid chromatography (HPLC/MS) has been used to analyse natural resins in ancient samples, particularly for paint varnishes containing mastic and dammar resins [34]. A partial limitation of chromatographic techniques is that they do not permit the analysis of the polymeric fraction or insoluble fraction that may be present in the native resins or formed in the course of ageing. Techniques based on the direct introduction of the sample in the mass spectrometer such as direct temperature resolved mass spectrometry (DTMS), direct exposure mass spectrometry (DE-MS) and direct inlet mass spectrometry (DI-MS), and on analytical pyrolysis (Py-GC/MS), have been employed as complementary techniques to obtain preliminary information on the... [Pg.217]

Identification and quantification of natural dyes need high performance analytical techniques, appropriate for the analysis of materials of complicated matrices containing a small amount of coloured substances. This requirement perfectly fits coupling of modern separation modules (usually high performance liquid chromatography in reversed phase mode, RPLC, but also capillary electrophoresis, CE) with selective detection units (mainly mass spectrometer). [Pg.365]

Consider one small molecule, phenylalanine. It is an essential amino acid in our diet and is important in protein synthesis (a component of protein), as well as a precursor to tyrosine and neurotransmitters. Phenylalanine is one of several amino acids that are measured in a variety of clinical methods, which include immunoassay, fluorometry, high performance liquid chromatography (HPLC see Section 4.1.2) and most recently MS/MS (see Chapter 3). Historically, screening labs utilized immunoassays or fluorimetric analysis. Diagnostic metabolic labs used the amino acid analyzer, which was a form of HPLC. Most recently, the tandem mass spectrometer has been used extensively in screening labs to analyze amino acids or in diagnostic labs as a universal detector for GC and LC techniques. Why did MS/MS replace older technological systems The answer to this question lies in the power of mass spectrometer. [Pg.289]

T. Storm, C. Hartig, T. Reemtsma and M. Jekel, Exact mass measurements on-line with high-performance liquid chromatography on a quadrupole mass spectrometer. Anal. Chem., 73 (2001) 589-595. [Pg.570]

A gas chromatograph with a capillary column coupled to a mass spectrometer is an ideal analytical partnership. Effluent from the column has an elevated temperature and the molecules of interest are in a vapor state and ready to enter the ion source. This eliminates the need for desolvation that is required in high-performance liquid chromatography (HPLC)-MS. [Pg.157]

It is now common to couple an instrument for separating a mixture of organic compounds e.g. using gas chromatography (GC) or high performance liquid chromatography (HPLC), directly to the input of a mass spectrometer. In this way, as each individual compound is separated from the mixture, its mass spectrum can be recorded and compared automatically with the library of known compounds and identified immediately if it is a known compound. [Pg.28]

The amount of cresol in the concentrated extract can then be determined by high performance liquid chromatography (HPLC) (DeRosa et al. 1987 Yoshikawa et al. 1986) or gas chromatography (GC) coupled to either a flame ionization detector (FID) or a mass spectrometer detection system (Angerer 1985 Needham et al. 1984). Separation of the cresol isomers by gas chromatography is readily accomplished, and the use of an appropriate internal standard allows the determination of their concentrations. Although exact detection limits were not given for the above GC methods, a concentration of 10 ppm appears to be readily determined. [Pg.131]

D Commercial COTS controlled by external computer Hybrid systems such as automated dissolution workstation with high-performance liquid chromatography (HPLC) or ultraviolet-visible (UV-Vis) interface Liquid chromatographs, gas chromatographs, UV/Vis spectrophotometers, Fourier transform infrared (FTIR) spectrophotometers, near-infrared (NIR) spectrophotometers, mass spectrometers, atomic absorption spectrometers, thermal gravimetric analyzers, COTS automation workstations... [Pg.793]

The availability of stable isotope-labeled PA makes an accurate quantitative determination of this imino acid possible. A short high-performance liquid chromatography (HPLC) run prior to the mass spectrometer inlet will result in a discrete peak of PA. For the definitive diagnosis of AASA dehydrogenase deficiency, a simultaneous determination of AASA would be preferred. The absence of a commercially available labeled standard leaves this analysis in the experimental stage. [Pg.130]

Superior sensitivity, efficiency, and specificity have made high-performance liquid chromatography coupled with tandem mass spectrometry (HPLC-MS/MS), the predominant analytical technique for characterization and quantitative analysis of metabolites (Kostiainen et al., 2003 Ma et al., 2006 Prakash et al., 2007). Ion trap, triple-quadrupole, and quadmpole time-of-flight (Q-TOF) mass spectrometers are routinely used to profile and characterize metabolites in plasma and excreta (Ma et al., 2006). The combination of scan types and features available on mass spectrometers of different design (product ion, MS", neutral loss, precursor ion scans, accurate mass measurements) allows identification and characterization of putative and unexpected metabolites with or without little prior knowledge of biotransformation pathways of a given dmg molecule. [Pg.296]

Rottmann, L. and Heumann, K.G. (1994) Determination of heavy metal interactions with dissolved organic materials in natural aquatic systems by coupling a high-performance liquid chromatography system with an inductively coupled plasma mass spectrometer. Anal. Chem., 66, 3709—3715. [Pg.231]


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See also in sourсe #XX -- [ Pg.207 , Pg.209 ]




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