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Start Over Descriptor "HILIC-MS/MS" Publication Type Electronic Resources
5 results on '"HILIC-MS/MS"'

1. Beta-N-Methylamino-L-Alanine: LC-MS/MS Optimization, Screening of Cyanobacterial Strains and Occurrence in Shellfish from Thau, a French Mediterranean Lagoon

Author

Reveillon, Damien, Abadie, Eric, Sechet, Veronique, Brient, Luc, Savar, Veronique, Bardouil, Michele, Hess, Philipp, Amzil, Zouher, Reveillon, Damien, Abadie, Eric, Sechet, Veronique, Brient, Luc, Savar, Veronique, Bardouil, Michele, Hess, Philipp, and Amzil, Zouher

Abstract

beta-N-methylamino-L-alanine (BMAA) is a neurotoxic non-protein amino acid suggested to be involved in neurodegenerative diseases. It was reported to be produced by cyanobacteria, but also found in edible aquatic organisms, thus raising concern of a widespread human exposure. However, the chemical analysis of BMAA and its isomers are controversial, mainly due to the lack of selectivity of the analytical methods. Using factorial design, we have optimized the chromatographic separation of underivatized analogues by a hydrophilic interaction chromatography coupled to tandem mass spectrometry (HILIC-MS/MS) method. A combination of an effective solid phase extraction (SPE) clean-up, appropriate chromatographic resolution and the use of specific mass spectral transitions allowed for the development of a highly selective and sensitive analytical procedure to identify and quantify BMAA and its isomers (in both free and total form) in cyanobacteria and mollusk matrices (LOQ of 0.225 and 0.15 mu g/g dry weight, respectively). Ten species of cyanobacteria (six are reported to be BMAA producers) were screened with this method, and neither free nor bound BMAA could be found, while both free and bound DAB were present in almost all samples. Mussels and oysters collected in 2009 in the Thau Lagoon, France, were also screened, and bound BMAA and its two isomers, DAB and AEG, were observed in all samples (from 0.6 to 14.4 mu g/g DW), while only several samples contained quantifiable free BMAA.

Published
2014
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2. Beta-N-Methylamino-L-Alanine: LC-MS/MS Optimization, Screening of Cyanobacterial Strains and Occurrence in Shellfish from Thau, a French Mediterranean Lagoon

Author

Reveillon, Damien, Abadie, Eric, Sechet, Veronique, Brient, Luc, Savar, Veronique, Bardouil, Michele, Hess, Philipp, Amzil, Zouher, Reveillon, Damien, Abadie, Eric, Sechet, Veronique, Brient, Luc, Savar, Veronique, Bardouil, Michele, Hess, Philipp, and Amzil, Zouher

Abstract

beta-N-methylamino-L-alanine (BMAA) is a neurotoxic non-protein amino acid suggested to be involved in neurodegenerative diseases. It was reported to be produced by cyanobacteria, but also found in edible aquatic organisms, thus raising concern of a widespread human exposure. However, the chemical analysis of BMAA and its isomers are controversial, mainly due to the lack of selectivity of the analytical methods. Using factorial design, we have optimized the chromatographic separation of underivatized analogues by a hydrophilic interaction chromatography coupled to tandem mass spectrometry (HILIC-MS/MS) method. A combination of an effective solid phase extraction (SPE) clean-up, appropriate chromatographic resolution and the use of specific mass spectral transitions allowed for the development of a highly selective and sensitive analytical procedure to identify and quantify BMAA and its isomers (in both free and total form) in cyanobacteria and mollusk matrices (LOQ of 0.225 and 0.15 mu g/g dry weight, respectively). Ten species of cyanobacteria (six are reported to be BMAA producers) were screened with this method, and neither free nor bound BMAA could be found, while both free and bound DAB were present in almost all samples. Mussels and oysters collected in 2009 in the Thau Lagoon, France, were also screened, and bound BMAA and its two isomers, DAB and AEG, were observed in all samples (from 0.6 to 14.4 mu g/g DW), while only several samples contained quantifiable free BMAA.

Published
2014
Full Text
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3. Beta-N-Methylamino-L-Alanine: LC-MS/MS Optimization, Screening of Cyanobacterial Strains and Occurrence in Shellfish from Thau, a French Mediterranean Lagoon

Author

Reveillon, Damien, Abadie, Eric, Sechet, Veronique, Brient, Luc, Savar, Veronique, Bardouil, Michele, Hess, Philipp, Amzil, Zouher, Reveillon, Damien, Abadie, Eric, Sechet, Veronique, Brient, Luc, Savar, Veronique, Bardouil, Michele, Hess, Philipp, and Amzil, Zouher

Abstract

beta-N-methylamino-L-alanine (BMAA) is a neurotoxic non-protein amino acid suggested to be involved in neurodegenerative diseases. It was reported to be produced by cyanobacteria, but also found in edible aquatic organisms, thus raising concern of a widespread human exposure. However, the chemical analysis of BMAA and its isomers are controversial, mainly due to the lack of selectivity of the analytical methods. Using factorial design, we have optimized the chromatographic separation of underivatized analogues by a hydrophilic interaction chromatography coupled to tandem mass spectrometry (HILIC-MS/MS) method. A combination of an effective solid phase extraction (SPE) clean-up, appropriate chromatographic resolution and the use of specific mass spectral transitions allowed for the development of a highly selective and sensitive analytical procedure to identify and quantify BMAA and its isomers (in both free and total form) in cyanobacteria and mollusk matrices (LOQ of 0.225 and 0.15 mu g/g dry weight, respectively). Ten species of cyanobacteria (six are reported to be BMAA producers) were screened with this method, and neither free nor bound BMAA could be found, while both free and bound DAB were present in almost all samples. Mussels and oysters collected in 2009 in the Thau Lagoon, France, were also screened, and bound BMAA and its two isomers, DAB and AEG, were observed in all samples (from 0.6 to 14.4 mu g/g DW), while only several samples contained quantifiable free BMAA.

Published
2014
Full Text
View/download PDF

4. Development and validation of a fast quantitative method for plasma dimethylarginines analysis using liquid chromatography-tandem mass spectrometry

Author

D'Apolito, O, Paglia, G, Tricarico, F, Garofalo, D, Pilotti, A, Lamacchia, O, Cignarelli, M, Corso, G, D'Apolito O., Paglia G., Tricarico F., Garofalo D., Pilotti A., Lamacchia O., Cignarelli M., Corso G., D'Apolito, O, Paglia, G, Tricarico, F, Garofalo, D, Pilotti, A, Lamacchia, O, Cignarelli, M, Corso, G, D'Apolito O., Paglia G., Tricarico F., Garofalo D., Pilotti A., Lamacchia O., Cignarelli M., and Corso G.

Abstract

Objectives: The aim of this work was to implement a fast, accurate and simple method to quantify plasma ADMA and SDMA, in a run time suitable for routine analysis. Design and methods: We developed and validated a hydrophilic interaction chromatographic method coupled to tandem mass spectrometry (HILIC-MS/MS) for separation and simultaneous quantification of Arginine (Arg) and its dimethylarginines, ADMA and SDMA, with a short run time (less than 5 min) using a small volume of human plasma (0.02 mL). Results: Correlation coefficients (r) of the calibration curves ranged from 0.9926 to 0.9984. Within-day and between-day imprecision (CV%) and inaccuracy (%), carry-over and recovery were also evaluated for validation. Preliminary data of Arg, ADMA and SDMA from 30 apparently healthy subjects and type 2 diabetic patients (n = 33) with and without kidney dysfunction were calculated and some statistical differences occurred among them (p < 0.05). Conclusions: Data from calibration curves and quality controls reveal that the method is accurate and precise. Healthy subjects and diabetic patients' values are in agreement with those reported in other studies. © 2008 The Canadian Society of Clinical Chemists

Published
2008

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