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Amino acids separation mass spectrometry detection

Mass spectrometry (MS) is also being used to add another dimension of analysis to achiral-chiral analysis. Recently, an achiral-chiral column-switching LC/LC-MS/MS method was reported for the pindolol enantiomers in human serum (Motoyama et al., 2002) and phenprocoumon metabolites (Kammerer et al., 1998). For analytes that have very poor chromophores or cannot naturally fluoresce, MS detection can be more sensitive for the underivatized form of the analyte. Also, MS detection can be particularly useful when very similar analytes that differ in mass (such as some amino acids and metabolites) cannot be satisfactorily separated chromatographically,... [Pg.324]

Determination of oxidized amino acids in urine is usually performed by isotope dilution gas chromatography-mass spectrometry (L9). DOPA is estimated by HPLC separation of acid protein hydrolysates with fluorescence detection (excitation 280 nm, emission at 320 nm) (A15). Other methods are based on borate-hydrochloric acid difference spectroscopy (this method suffers interference from tyrosine and tryptophan) (W2), derivatization of DOPA with nitrite and subsequent coulometric determination (W3), and fluorometric detection after derivatization with ethylenediamine (A15). 3-Hydroxylysine is quantitated by HPLC with 9-fluorenylmethyl chloroformate precolumn derivatization (M25) of amino acids obtained by gas-phase hydrolysis of proteins (F21). Other general methods to detect amino acid damage are mass spectometry methods applied to protein hydrolysates, such as tandem mass spectrometry (F6). [Pg.229]

UV and fluorescent spectroscopy can be employed down to 190 nm because there is no solvent interference. Mass spectrometry is easy because the water provides good ionization. Flame ionization detection (FID) is of particular interest because potentially it offers a sensitive and universal detector. A number of different interfaces have been used, including heated capillaries, which have been examined by Miller and Hawthorne [62], Ingelse et al. [63], and others [64, 65], who separated a range of analytes including alcohols, amino acids, and phenols. An alternative method employing a cold nebuliza-tion of the eluent has been introduced by Bone et al. [66]. They were able to detect both aliphatic and aromatic alcohols, polymers, carbohydrates, parabens, and steroids. [Pg.824]

New methods use combined HPLC/Mass spectrometry to identify modified amino acids. Purified recombinant human insulin-like growth factor separated into two peaks on reverse phase HPLC (Cl 8 column/acidified water) even though other methods indicated it was completely pure. Plasma desorption mass spectrometry of the individual peptides detected a single methionine sulfoxide molecule that was sufficient to decrease the hydrophobicity of the whole protein significantly. Most of the oxidation occurred when the secreted fusion protein was cleaved with hydroxylamine under not strictly anaerobic conditions, but about 5% occurred during die . coli fermentation. [Pg.31]

GC-MS Gas chromatography-mass spectrometry is the most versatile method. It can be used for pyrolysates (see above), but also for the detection of PAHs in extracts. In combination with commercially available derivatization protocols, amino acids can be analyzed as well. If chiral columns are used, enantiomeric separation of chiral compounds is possible. Usually, either quadrupole or ion trap mass spectrometers are used as detectors, but Time-of-flight (ToF) MS can also be used. [Pg.252]

The isolation and identification of the light, acid, and base sensitive musca-aurins posed considerable separation problems which were overcome by careful, repeated chromatography on Sephadex 188, 192). Hydrolysis of the individual musca-aurins gave betalamic acid (174) together with the constituent amino acids which were detected by electrophoresis and paper chromatography and identified by linked gas chromatography-mass spectrometry of their 7V-trifluoroacetyl methyl esters 189,192). [Pg.79]


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