Your search keyword '"Bouatra S"' showing total 10 results

1. A metabolomics approach to uncover the effects of grain diets on rumen health in dairy cows

Author

Saleem, F., Ametaj, B.N., Bouatra, S., Mandal, R., Zebeli, Q., Dunn, S.M., and Wishart, D.S.

Published

2012

2. HMDB: A knowledgebase for the human metabolome

Author

Lewis, A., Wishart, D.S., Guo, A.C., Gautam, B., Tzur, D., Sobsey, C.A., Shaykhutdinov, R., Fradette, R., De Souza, A., Cruz, J.A., Xiong, Y., Bouatra, S., Mandal, R., Psychogios, N., Sinelnikov, I., Vogel, H.J., Fang, L., Peng, J., Xia, J., Li, L., Knox, C., Shrivastava, S., Clements, M., Lim, E., Eisner, R., Cheng, D., Dawe, M., Zuniga, A., Young, N., Jia, L., Grenier, R., Hau, D.D., Huang, P., Nazyrova, A., Liu, P., Forsythe, I., Dong, E., and Clive, D.

Published

2009

3. HMDB: a knowledgebase for the human metabolome

Author

Wishart, D. S., primary, Knox, C., additional, Guo, A. C., additional, Eisner, R., additional, Young, N., additional, Gautam, B., additional, Hau, D. D., additional, Psychogios, N., additional, Dong, E., additional, Bouatra, S., additional, Mandal, R., additional, Sinelnikov, I., additional, Xia, J., additional, Jia, L., additional, Cruz, J. A., additional, Lim, E., additional, Sobsey, C. A., additional, Shrivastava, S., additional, Huang, P., additional, Liu, P., additional, Fang, L., additional, Peng, J., additional, Fradette, R., additional, Cheng, D., additional, Tzur, D., additional, Clements, M., additional, Lewis, A., additional, De Souza, A., additional, Zuniga, A., additional, Dawe, M., additional, Xiong, Y., additional, Clive, D., additional, Greiner, R., additional, Nazyrova, A., additional, Shaykhutdinov, R., additional, Li, L., additional, Vogel, H. J., additional, and Forsythe, I., additional

Published

2009

4. Efficiency of Dinucleosides as the Backbone to Pre-Organize Multi-Porphyrins and Enhance Their Stability as Sandwich Type Complexes with DABCO.

Author

Merkaš S, Bouatra S, Rein R, Piantanida I, Zinic M, and Solladié N

Subjects

Dimerization, Kinetics, Piperazines chemical synthesis, Porphyrins chemical synthesis, Spectrophotometry, Ultraviolet, Nucleosides chemistry, Piperazines chemistry, Porphyrins chemistry

Abstract

Flexible linkers such as uridine or 2'-deoxyuridine pre-organize bis-porphyrins in a face-to-face conformation, thus forming stable sandwich complexes with a bidentate base such as 1,4-diazabicyclo[2.2.2]octane (DABCO). Increased stability can be even greater when a dinucleotide linker is used. Such pre-organization increases the association constant by one to two orders of magnitude when compared to the association constant of DABCO with a reference porphyrin. Comparison with rigid tweezers shows a better efficiency of nucleosidic dimers. Thus, the choice of rigid spacers is not the only way to pre-organize bis-porphyrins, and well-chosen nucleosidic linkers offer an interesting option for the synthesis of such devices., Competing Interests: The authors declare no conflict of interest.

Published

2017

5. High Field Solid-State NMR Spectroscopy Investigation of (15)N-Labeled Rosette Nanotubes: Hydrogen Bond Network and Channel-Bound Water.

Author

Fenniri H, Tikhomirov GA, Brouwer DH, Bouatra S, El Bakkari M, Yan Z, Cho JY, and Yamazaki T

Abstract

(15)N-labeled rosette nanotubes were synthesized and investigated using high-field solid-state NMR spectroscopy, X-ray diffraction, atomic force microscopy, and electron microscopy. The results established the H-bond network involved in the self-assembly of the nanostructure as well as bound water molecules in the nanotube's channel.

Published

2016

6. Metabolomic fingerprint of heart failure with preserved ejection fraction.

Author

Zordoky BN, Sung MM, Ezekowitz J, Mandal R, Han B, Bjorndahl TC, Bouatra S, Anderson T, Oudit GY, Wishart DS, and Dyck JR

Subjects

Aged, Case-Control Studies, Demography, Female, Heart Failure blood, Humans, Male, Metabolome, Middle Aged, Natriuretic Peptide, Brain blood, Peptide Fragments blood, Peptides blood, ROC Curve, Heart Failure metabolism, Heart Failure physiopathology, Metabolomics, Stroke Volume

Abstract

Background: Heart failure (HF) with preserved ejection fraction (HFpEF) is increasingly recognized as an important clinical entity. Preclinical studies have shown differences in the pathophysiology between HFpEF and HF with reduced ejection fraction (HFrEF). Therefore, we hypothesized that a systematic metabolomic analysis would reveal a novel metabolomic fingerprint of HFpEF that will help understand its pathophysiology and assist in establishing new biomarkers for its diagnosis., Methods and Results: Ambulatory patients with clinical diagnosis of HFpEF (n = 24), HFrEF (n = 20), and age-matched non-HF controls (n = 38) were selected for metabolomic analysis as part of the Alberta HEART (Heart Failure Etiology and Analysis Research Team) project. 181 serum metabolites were quantified by LC-MS/MS and 1H-NMR spectroscopy. Compared to non-HF control, HFpEF patients demonstrated higher serum concentrations of acylcarnitines, carnitine, creatinine, betaine, and amino acids; and lower levels of phosphatidylcholines, lysophosphatidylcholines, and sphingomyelins. Medium and long-chain acylcarnitines and ketone bodies were higher in HFpEF than HFrEF patients. Using logistic regression, two panels of metabolites were identified that can separate HFpEF patients from both non-HF controls and HFrEF patients with area under the receiver operating characteristic (ROC) curves of 0.942 and 0.981, respectively., Conclusions: The metabolomics approach employed in this study identified a unique metabolomic fingerprint of HFpEF that is distinct from that of HFrEF. This metabolomic fingerprint has been utilized to identify two novel panels of metabolites that can separate HFpEF patients from both non-HF controls and HFrEF patients., Clinical Trial Registration: ClinicalTrials.gov NCT02052804.

Published

2015

7. The human urine metabolome.

Author

Bouatra S, Aziat F, Mandal R, Guo AC, Wilson MR, Knox C, Bjorndahl TC, Krishnamurthy R, Saleem F, Liu P, Dame ZT, Poelzer J, Huynh J, Yallou FS, Psychogios N, Dong E, Bogumil R, Roehring C, and Wishart DS

Subjects

Databases, Factual, Humans, Magnetic Resonance Spectroscopy, Metabolome, Urinalysis

Abstract

Urine has long been a "favored" biofluid among metabolomics researchers. It is sterile, easy-to-obtain in large volumes, largely free from interfering proteins or lipids and chemically complex. However, this chemical complexity has also made urine a particularly difficult substrate to fully understand. As a biological waste material, urine typically contains metabolic breakdown products from a wide range of foods, drinks, drugs, environmental contaminants, endogenous waste metabolites and bacterial by-products. Many of these compounds are poorly characterized and poorly understood. In an effort to improve our understanding of this biofluid we have undertaken a comprehensive, quantitative, metabolome-wide characterization of human urine. This involved both computer-aided literature mining and comprehensive, quantitative experimental assessment/validation. The experimental portion employed NMR spectroscopy, gas chromatography mass spectrometry (GC-MS), direct flow injection mass spectrometry (DFI/LC-MS/MS), inductively coupled plasma mass spectrometry (ICP-MS) and high performance liquid chromatography (HPLC) experiments performed on multiple human urine samples. This multi-platform metabolomic analysis allowed us to identify 445 and quantify 378 unique urine metabolites or metabolite species. The different analytical platforms were able to identify (quantify) a total of: 209 (209) by NMR, 179 (85) by GC-MS, 127 (127) by DFI/LC-MS/MS, 40 (40) by ICP-MS and 10 (10) by HPLC. Our use of multiple metabolomics platforms and technologies allowed us to identify several previously unknown urine metabolites and to substantially enhance the level of metabolome coverage. It also allowed us to critically assess the relative strengths and weaknesses of different platforms or technologies. The literature review led to the identification and annotation of another 2206 urinary compounds and was used to help guide the subsequent experimental studies. An online database containing the complete set of 2651 confirmed human urine metabolite species, their structures (3079 in total), concentrations, related literature references and links to their known disease associations are freely available at http://www.urinemetabolome.ca.

Published

2013

8. Differential metabolite profiles and salinity tolerance between two genetically related brown-seeded and yellow-seeded Brassica carinata lines.

Author

Canam T, Li X, Holowachuk J, Yu M, Xia J, Mandal R, Krishnamurthy R, Bouatra S, Sinelnikov I, Yu B, Grenkow L, Wishart DS, Steppuhn H, Falk KC, Dumonceaux TJ, and Gruber MY

Subjects

Adaptation, Physiological, Biofuels, Crops, Agricultural genetics, Crops, Agricultural metabolism, Gene Expression Regulation, Plant, Genetic Variation, Genotype, Phenotype, Pigmentation genetics, Salinity, Seeds genetics, Seeds metabolism, Stress, Physiological, Brassica genetics, Brassica metabolism, Salt-Tolerant Plants genetics, Salt-Tolerant Plants metabolism, Sulfates metabolism

Abstract

Brassica carinata (Ethiopian mustard) has previously been identified as a potential crop species suitable for marginal land in the North American prairies due to its relatively high salt tolerance. Two genetically related B. carinata lines with brown-seeded (BS) and yellow-seeded (YS) phenotypes were assessed for their tolerance to sodium sulfate. Specifically, each line was greenhouse-grown under 0, 50 and 100mM of salt, and analyzed after four weeks and eight weeks of treatment. Generally, the height of the BS line was greater than the YS line under both salt treatments, indicating enhanced salt tolerance of the BS line. NMR-based metabolite profiling and PCA analyses indicated a more pronounced shift in key stem metabolites after four weeks of treatment with the YS line compared to the BS line. For example, tryptophan and formate levels increased in the YS line after four weeks of 100mM salt treatment, while proline and threonine levels varied uniquely compared to other metabolites of the lines. Together, the data indicate that the brown-seeded line has greater sodium tolerance than the yellow-seed line, provide clues to the biochemical underpinnings for the phenotypic variation, and highlight the utility of B. carinata as a biorefinery crop for saline land., (Copyright © 2012 Elsevier Ireland Ltd. All rights reserved.)

Published

2013

9. HMDB 3.0--The Human Metabolome Database in 2013.

Author

Wishart DS, Jewison T, Guo AC, Wilson M, Knox C, Liu Y, Djoumbou Y, Mandal R, Aziat F, Dong E, Bouatra S, Sinelnikov I, Arndt D, Xia J, Liu P, Yallou F, Bjorndahl T, Perez-Pineiro R, Eisner R, Allen F, Neveu V, Greiner R, and Scalbert A

Subjects

Humans, Internet, Mass Spectrometry, Nuclear Magnetic Resonance, Biomolecular, User-Computer Interface, Databases, Chemical, Metabolome, Metabolomics

Abstract

The Human Metabolome Database (HMDB) (www.hmdb.ca) is a resource dedicated to providing scientists with the most current and comprehensive coverage of the human metabolome. Since its first release in 2007, the HMDB has been used to facilitate research for nearly 1000 published studies in metabolomics, clinical biochemistry and systems biology. The most recent release of HMDB (version 3.0) has been significantly expanded and enhanced over the 2009 release (version 2.0). In particular, the number of annotated metabolite entries has grown from 6500 to more than 40,000 (a 600% increase). This enormous expansion is a result of the inclusion of both 'detected' metabolites (those with measured concentrations or experimental confirmation of their existence) and 'expected' metabolites (those for which biochemical pathways are known or human intake/exposure is frequent but the compound has yet to be detected in the body). The latest release also has greatly increased the number of metabolites with biofluid or tissue concentration data, the number of compounds with reference spectra and the number of data fields per entry. In addition to this expansion in data quantity, new database visualization tools and new data content have been added or enhanced. These include better spectral viewing tools, more powerful chemical substructure searches, an improved chemical taxonomy and better, more interactive pathway maps. This article describes these enhancements to the HMDB, which was previously featured in the 2009 NAR Database Issue. (Note to referees, HMDB 3.0 will go live on 18 September 2012.).

Published

2013

10. The human serum metabolome.

Author

Psychogios N, Hau DD, Peng J, Guo AC, Mandal R, Bouatra S, Sinelnikov I, Krishnamurthy R, Eisner R, Gautam B, Young N, Xia J, Knox C, Dong E, Huang P, Hollander Z, Pedersen TL, Smith SR, Bamforth F, Greiner R, McManus B, Newman JW, Goodfriend T, and Wishart DS

Subjects

Adult, Aged, Blood Chemical Analysis methods, Blood Proteins analysis, Blood Proteins metabolism, Case-Control Studies, Databases, Protein, Female, Gas Chromatography-Mass Spectrometry, Health, Humans, Lipids analysis, Lipids blood, Male, Metabolomics methods, Middle Aged, Nuclear Magnetic Resonance, Biomolecular, Osmolar Concentration, Review Literature as Topic, Serum chemistry, Spectrometry, Mass, Electrospray Ionization, Metabolome physiology, Serum metabolism

Abstract

Continuing improvements in analytical technology along with an increased interest in performing comprehensive, quantitative metabolic profiling, is leading to increased interest pressures within the metabolomics community to develop centralized metabolite reference resources for certain clinically important biofluids, such as cerebrospinal fluid, urine and blood. As part of an ongoing effort to systematically characterize the human metabolome through the Human Metabolome Project, we have undertaken the task of characterizing the human serum metabolome. In doing so, we have combined targeted and non-targeted NMR, GC-MS and LC-MS methods with computer-aided literature mining to identify and quantify a comprehensive, if not absolutely complete, set of metabolites commonly detected and quantified (with today's technology) in the human serum metabolome. Our use of multiple metabolomics platforms and technologies allowed us to substantially enhance the level of metabolome coverage while critically assessing the relative strengths and weaknesses of these platforms or technologies. Tables containing the complete set of 4229 confirmed and highly probable human serum compounds, their concentrations, related literature references and links to their known disease associations are freely available at http://www.serummetabolome.ca.

Published

2011