Project description:Exposome analysis in humans. Negative ion mode data. Reverse phase chromatography.

Project description:Wild type and creatine kinase knock-out mice were subjected to a multi-organ metabolomic and proteomics comparative analysis using a streamline sample preparation method which allowed both metabolite and proteomic analysis of each organ. The metabolites were spiked with an heavy internal reference metabolite standards and analyzed using optimized reverse phase HPLC analysis in both positive and negative mode on a Q Exactive Classic. A reference standard library consisting of over 600 reference metabolite standards were analyzed on this system for extra confidence in the identification and quantification of this library of key metabolites. This repository solely contains the metabolomic data. A second repository will contain the matched proteomic data.

Project description:Exposome analysis in humans. Negative ion mode data. Reverse phase chromatography.

Project description:Secondary metabolite profiles of Aspergillus fumigatus aneuploids, WT, and nscROE strains under FK506 stress. Data include both positive and negative ionization modes from a 25-minute reverse-phase run conducted in 2025.

Project description:<p>The totality of environmental exposures and lifestyle factors, commonly referred to as the exposome, are poorly understood. Measuring the myriad of chemicals that humans are exposed to is immensely challenging and identifying disrupted metabolic pathways is even more complex. Here, we present a novel technological approach for the comprehensive, rapid and integrated analysis of the endogenous human metabolome and the chemical exposome. By combining reverse-phase and hydrophilic interaction liquid chromatography and fast polarity switching, molecules with highly diverse chemical structures can be analyzed in 15 min with a single analytical run as both column’s effluents are combined before analysis. Standard reference materials and authentic standards were evaluated to critically benchmark performance. Highly sensitive median limits of detection (LOD) with 0.04 μM for &gt;140 quantitatively assessed endogenous metabolites and 0.08 ng/mL for the &gt;100 model xenobiotics and human estrogens in solvent were obtained. In matrix, the median LOD values were higher with 0.7 ng/mL (urine) and 0.5 ng/mL (plasma) for exogenous chemicals. To prove the dual-column approach’s applicability, real-life urine samples from sub-Saharan Africa (high exposure scenario) and Europe (low exposure scenario) were assessed in a targeted and non-targeted manner. Our LC-HRMS approach demonstrates the feasibility of quantitatively and simultaneously assessing the endogenous metabolome and the chemical exposome for the high-throughput measurement of environmental drivers of disease.</p>

Project description:Solanum is one of the most economically valuable genera in the Solanaceae family, covering cultivated vegetable crops, medicinal plants and wild germplasms, while systematic metabolomics reference datasets for diverse Solanum germplasms remain scarce. Here, we performed untargeted metabolomics profiling on fruit samples of three core Solanum germplasms: common cultivated eggplant S. melongena, S. undatum, S. aethiopicum, with 6 biological replicates for each germplasm grown under uniform field conditions. Standard sample pretreatment and downstream analyses (repeatability test, PCA, differential metabolite screening and KEGG pathway enrichment analysis) were conducted. KEGG enrichment analysis (VIP > 1, P < 0.05) revealed that biosynthesis of amino acids and cofactors was the core pathway driving metabolic differentiation under both ionization modes. Stress-related secondary metabolic pathways were exclusively enriched in positive ionization mode, while galactose and carbon metabolism were significantly enriched in negative ionization mode. Collectively, metabolic variations among the three germplasms mainly concentrated in amino acid and cofactor pathways, coupled with stress-related secondary metabolism in positive mode and sugar/carbon metabolism in negative mode.

Project description:analysis of drugs from the dark web. analyzed by positive and negative mode electrospray ionization. UPHLC-MS. reverse-phase chromatography (C18).

Project description:UHPLC-HRMS/MS data of murine colon tissue in positive and negative mode. Metabolomics. Reverse phase chromatography using F5 column. Iterative DDA data collected using AcquireX procedure on Thermo MS.

Project description:The global proteome analysis was limited by the identification of peptides with low abundance or specific physiochemical properties. Here, a one-dimensional online alkaline-pH reverse phase nanoelectrospray-tandem mass spectrometry (AlkalinepH-MS/MS) method was developed and optimized for global proteomic analysis. In this method, peptides were separated on a nanoflow C18 column with an alkaline-pH mobile phase (pH=8) and directly introduced to the mass spectrometer through nanoelectrospray ionization. The identified peptides overlapped between AlkalinepH-MS/MS and conventional online low-pH reverse phase nanoelectrospray-tandem mass spectrometry (LowpH-MS/MS) were as low as 45%, indicating that these two methods were complementary to each other. In addition, the AlkalinepH-MS/MS method showed identification capacity for a higher proportion of peptides with low molecular weight (MW), positive grand average of hydropathy (GRAVY), or high isoelectric point (pI). Moreover, the AlkalinepH-MS/MS method had a bias toward histidine, lysine, methionine, and proline- containing peptides. The complementarity of AlkalinepH-MS/MS and LowpH-MS/MS was further demonstrated for the analysis of tryptic digests from 15 intrahepatic cholangiocarcinoma (iCCA) cell lines. The alternating of 60-min AlkalinepH-MS/MS and 60-min LowpH-MS/MS method outperformed the conventional 120-min LowpH-MS/MS method in the identification of amino acid variants and protein groups. Our AlkalinepH-MS/MS method was an excellent complementary and alternative method to the LowpH-MS/MS method for global proteomic analysis.

Project description:Data used in the creation of the Baker Lab PFAS LC-IMS-MS Skyline Library as of 10/2024. Includes reversed-phase liquid chromatography retention times, collision cross section (CCS) values, and m/z ratios for 174 PFAS and their resulting 280 ion types in positive and negative modes with electrospray ionization (ESI) and atmospheric pressure chemical ionization (APCI) sources. To use, please select the sheet which most accurately reflects your ionization method and mode, then copy and paste columns B-G, including column headers listed in row 4.