HMDB: a knowledgebase for the human metabolome

Wishart, David S.; Knox, Craig; Guo, Anchi; Eisner, Roman; Young, Nelson D.; Gautam, Bijaya; Hau, David; Psychogios, Nikolaos; Dong, Erbao; Bouatra, Souhaila; Mandal, Rupasri; Sinelnikov, Igor; Xia, Jianguo; Jia, Leslie; Cruz, Joseph A.; Lim, Emilia L.; Sobsey, Constance A.; Shrivastava, Savita; Huang, Paul H.; Liu, Philip L.‐F.; Fang, Lydia; Peng, Jun; Fradette, Ryan; Cheng, Dongping; Tzur, Dan; Clements, Melisa; Lewis, Avalyn; Souza, Andrea De; Zuniga, Azaret; Dawe, Margot; Xiong, Yeping; Clive, Derrick L. J.; Greiner, Russell; Nazyrova, Alsu; Shaykhutdinov, Rustem; Li, Liang; Vogel, Hans J.; Forsythe, Ian J.

doi:10.1093/nar/gkn810

Cited by 1,682 publications

(1,353 citation statements)

References 25 publications

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“…The results of our accurate mass measurements annotated in Figure 1B agree with previously published data from isotope labeling studies carried out on U [16]. We have reinterpreted this labeling data, which was originally only discussed in terms of 15 N, 13 C, and 18 O labeling [16], to include the results from dissociation of [5,6-D 2 ]uracil that had not previously been explained but are critical in explaining several dissociation pathways. Based on this interpretation, the composition and atom position of each product-ion and all neutral losses are presented in Table 1, which is the starting point for our spectral interpretation.…”

Section: Resultssupporting

confidence: 85%

“…Such de novo identification aims to correlate observed spectral features in MS/MS to the structures of investigated species based on established reactivity for a class of compounds [4,[6][7][8][9]. The idea of using MS/MS as stand-alone identification tool is of increasing interest and is also being addressed using other more general approaches intended to generalize dissociation pathways [10], to automate data analysis [11], or to compile spectra in databases [12,13].…”

Section: Introductionmentioning

confidence: 99%

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Revisiting the Reactivity of Uracil During Collision Induced Dissociation: Tautomerism and Charge-Directed Processes

Beach

Gabryelski

2012

J. Am. Soc. Mass Spectrom.

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In our recent work towards the nontarget identification of products of nucleic acid (NA) damage in urine, we have found previous work describing the dissociation of NA bases not adequate to fully explain their observed reactivity. Here we revisit the gas-phase chemistry of protonated uracil (U) during collision induced dissociation (CID) using two modern tandem mass spectrometry techniques; quadrupole ion trap (QIT) and quadrupole time of flight (Q-TOF). We present detailed mechanistic proposals that account for all observed products of our experiments and from previous isotope labeling data, and that are supported by previous ion spectroscopy results and theoretical work. The diverse product-ions of U cannot be explained adequately by only considering the lowest energy form of protonated U as a precursor. The tautomers adopted by U during collisional excitation make it possible to relate the complex reactivity observed to reasonable mechanistic proposals and feasible product-ion structures for this small highly conjugated heterocycle. These reactions proceed from four different stable tautomers, which are excited to a specific activated precursor from which dissociation can occur via a charge-directed process through a favorable transition state to give a stabilized product. Understanding the chemistry of uracil at this level will facilitate the identification of new modified uracil derivatives in biological samples based solely on their reactivity during CID. Our integrated approach to describing ion dissociation is widely applicable to other NA bases and similar classes of biomolecules.

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Section: Resultssupporting

confidence: 85%

Section: Introductionmentioning

confidence: 99%

Revisiting the Reactivity of Uracil During Collision Induced Dissociation: Tautomerism and Charge-Directed Processes

Beach

Gabryelski

2012

J. Am. Soc. Mass Spectrom.

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“…all metabolites will be detected once they are present in concentrations above the limit of detection. Two-dimensional (2D) NMR experiments such as TOCSY, 1 H J-RES and 1 H- 13 C HSQC are important to use in conjunction with one-dimensional spectra for metabolite identification (21) and to compare with reference databases such as the Human Metabolome Database (22) and Biological Magnetic Resonance Databank (23) . In addition, one-dimensional and 2D NMR experiments offer the potential to identify previously unknown metabolites (24) .…”

Section: Nmr Spectroscopymentioning

confidence: 99%

The role of metabolomics in determination of new dietary biomarkers

O’Gorman

Brennan

2017

Proc. Nutr. Soc.

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Traditional methods for the assessment of dietary intake are prone to error; in order to improve and enhance these methods increasing interest in the identification of dietary biomarkers has materialised. Metabolomics has emerged as a key tool in the area of dietary biomarker discovery and to date the use of metabolomics has identified a number of putative biomarkers. Applications to identify novel biomarkers of intake have in general taken three approaches: (1) specific acute intervention studies to identify specific biomarkers of intake; (2) searching for biomarkers in cohort studies by correlating to self-reported intake of a specific food/food group(s); (3) analysing dietary patterns in conjunction with metabolomic profiles to identify biomarkers and nutritypes. A number of analytical technologies are employed in metabolomics as currently there is no single technique capable of measuring the entire metabolome. These approaches each have their own advantages and disadvantages. The present review will provide an overview of current technologies and applications of metabolomics in the determination of new dietary biomarkers. In addition, it will address some of the current challenges in the field and future outlooks.

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“…The detected ion pairs can be searched against a database for putative metabolite identification or a library of standards for definitive identification. In this work, putative identification is based on the accurate mass matches of the dansylated metabolites with the human endogenous metabolites found in the Human Metabolome Database (HMDB) (about 8000 metabolite entries) [30]. Definitive identification is based on matches of accurate masses and retention times to a 13 C-/ 12 C-labeled authentic standards library (220 standards; see below).…”

Section: Lc-fticr Ms Measurementmentioning

confidence: 99%

Qualitative Metabolome Analysis of Human Cerebrospinal Fluid by¹³C-/¹²C-Isotope Dansylation Labeling Combined with Liquid Chromatography Fourier Transform Ion Cyclotron Resonance Mass Spectrometry

Guo

Bamforth

2011

J. Am. Soc. Mass Spectrom.

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Metabolome analysis of human cerebrospinal fluid (CSF) is challenging because of low abundance of metabolites present in a small volume of sample. We describe and apply a sensitive isotope labeling LC-MS technique for qualitative analysis of the CSF metabolome. After a CSF sample is divided into two aliquots, they are labeled by 13 C-dansyl and 12 C-dansyl chloride, respectively. The differentially labeled aliquots are then mixed and subjected to LC-MS using Fourier-transform ion cyclotron resonance mass spectrometry (FTICR MS). Dansylation offers significant improvement in the performance of chromatography separation and detection sensitivity. Moreover, peaks detected in the mass spectra can be readily analyzed for ion pair recognition and database search based on accurate mass and/or retention time information. It is shown that about 14,000 features can be detected in a 25-min LC-FTICR MS run of a dansyl-labeled CSF sample, from which about 500 metabolites can be profiled. Results from four CSF samples are compared to gauge the detectability of metabolites by this method. About 261 metabolites are commonly detected in replicate runs of four samples. In total, 1132 unique metabolite ion pairs are detected and 347 pairs (31%) matched with at least one metabolite in the Human Metabolome Database. We also report a dansylation library of 220 standard compounds and, using this library, about 85 metabolites can be positively identified. Among them, 21 metabolites have never been reported to be associated with CSF. These results illustrate that the dansylation LC-FTICR MS method can be used to analyze the CSF metabolome in a more comprehensive manner.

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HMDB: a knowledgebase for the human metabolome

Cited by 1,682 publications

References 25 publications

Revisiting the Reactivity of Uracil During Collision Induced Dissociation: Tautomerism and Charge-Directed Processes

Revisiting the Reactivity of Uracil During Collision Induced Dissociation: Tautomerism and Charge-Directed Processes

The role of metabolomics in determination of new dietary biomarkers

Qualitative Metabolome Analysis of Human Cerebrospinal Fluid by¹³C-/¹²C-Isotope Dansylation Labeling Combined with Liquid Chromatography Fourier Transform Ion Cyclotron Resonance Mass Spectrometry

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HMDB: a knowledgebase for the human metabolome

Cited by 1,682 publications

References 25 publications

Revisiting the Reactivity of Uracil During Collision Induced Dissociation: Tautomerism and Charge-Directed Processes

Revisiting the Reactivity of Uracil During Collision Induced Dissociation: Tautomerism and Charge-Directed Processes

The role of metabolomics in determination of new dietary biomarkers

Qualitative Metabolome Analysis of Human Cerebrospinal Fluid by13C-/12C-Isotope Dansylation Labeling Combined with Liquid Chromatography Fourier Transform Ion Cyclotron Resonance Mass Spectrometry

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Product

Resources

About

Qualitative Metabolome Analysis of Human Cerebrospinal Fluid by¹³C-/¹²C-Isotope Dansylation Labeling Combined with Liquid Chromatography Fourier Transform Ion Cyclotron Resonance Mass Spectrometry