Summary of Study ST002359

This data is available at the NIH Common Fund's National Metabolomics Data Repository (NMDR) website, the Metabolomics Workbench, https://www.metabolomicsworkbench.org, where it has been assigned Project ID PR001514. The data can be accessed directly via it's Project DOI: 10.21228/M80H6B This work is supported by NIH grant, U2C- DK119886.

See: https://www.metabolomicsworkbench.org/about/howtocite.php

This study contains a large results data set and is not available in the mwTab file. It is only available for download via FTP as data file(s) here.

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Study ID	ST002359
Study Title	Effect of hypoxia and reoxygenation on the adult hooded seal brain lipidome
Study Summary	Brain samples from adult hooded seals (Cystophora cristata) were subjected to hypoxia and reoxygenation in vitro and lipid composition was compared.
Institute	University of Hamburg
Last Name	Martens
First Name	Gerrit Alexander
Address	Martin-Luther-King-Platz 3, 20146 Hamburg, Germany
Email	gerrit.alexander.martens@uni-hamburg.de
Phone	+49 40 42838-3934
Submit Date	2022-11-23
Raw Data Available	Yes
Raw Data File Type(s)	cdf
Analysis Type Detail	LC-MS
Release Date	2023-04-12
Release Version	1

Select appropriate tab below to view additional metadata details:

Project:

Project ID:	PR001514
Project DOI:	doi: 10.21228/M80H6B
Project Title:	Lipidomics of deep-diving pinniped brains
Project Summary:	The brain of diving mammals such as the hooded seal (Cystophora cristata) exhibits a remarkable tolerance to low tissue oxygen levels (hypoxia). While neurons of most terrestrial mammals suffer irreversible damage after only short periods of hypoxia, in vitro experiments revealed that neurons of the hooded seal show prolonged functional integrity even in severe hypoxia. As major components of membranes, specific neuronal lipids of diving mammals could contribute to the observed high hypoxia tolerance. Therefore, we analyzed the brain lipidome of deep-diving pinnipeds (Cystophora cristata, Pagophilus groenlandicus) in comparison to terrestrial (non-diving) relatives (Mustela putorius furo, Mus musculus). Furthermore, lipid composition of C. cristata brain tissue was analyzed that was exposed to hypoxia and reoxygenation in vitro.
Institute:	University of Hamburg
Last Name:	Martens
First Name:	Gerrit Alexander
Address:	Martin-Luther-King-Platz 3, 20146 Hamburg, Germany
Email:	gerrit.alexander.martens@uni-hamburg.de
Phone:	+49 40 42838-3934

Subject:

Subject ID:	SU002448
Subject Type:	Mammal
Subject Species:	Cystophora cristata

Factors:

Subject type: Mammal; Subject species: Cystophora cristata (Factor headings shown in green)

mb_sample_id	local_sample_id	species	age	brain region	treatment	replicate
SA236964	Ccr2-1_VC_HO	Cystophora cristata	adult	visual cortex	hypoxia	1
SA236965	Ccr4-1_VC_HO	Cystophora cristata	adult	visual cortex	hypoxia	1
SA236966	Ccr1-1_VC_HO	Cystophora cristata	adult	visual cortex	hypoxia	1
SA236967	Ccr3-1_VC_HO	Cystophora cristata	adult	visual cortex	hypoxia	1
SA236968	Ccr2-2_VC_HO	Cystophora cristata	adult	visual cortex	hypoxia	2
SA236969	Ccr1-2_VC_HO	Cystophora cristata	adult	visual cortex	hypoxia	2
SA236970	Ccr3-2_VC_HO	Cystophora cristata	adult	visual cortex	hypoxia	2
SA236971	Ccr4-2_VC_HO	Cystophora cristata	adult	visual cortex	hypoxia	2
SA236972	Ccr1-3_VC_HO	Cystophora cristata	adult	visual cortex	hypoxia	3
SA236973	Ccr2-3_VC_HO	Cystophora cristata	adult	visual cortex	hypoxia	3
SA236974	Ccr4-3_VC_HO	Cystophora cristata	adult	visual cortex	hypoxia	3
SA236975	Ccr3-3_VC_HO	Cystophora cristata	adult	visual cortex	hypoxia	3
SA236976	Ccr4-1_VC_NO	Cystophora cristata	adult	visual cortex	normoxia	1
SA236977	Ccr1-1_VC_NO	Cystophora cristata	adult	visual cortex	normoxia	1
SA236978	Ccr2-1_VC_NO	Cystophora cristata	adult	visual cortex	normoxia	1
SA236979	Ccr3-1_VC_NO	Cystophora cristata	adult	visual cortex	normoxia	1
SA236980	Ccr2-2_VC_NO	Cystophora cristata	adult	visual cortex	normoxia	2
SA236981	Ccr4-2_VC_NO	Cystophora cristata	adult	visual cortex	normoxia	2
SA236982	Ccr1-2_VC_NO	Cystophora cristata	adult	visual cortex	normoxia	2
SA236983	Ccr3-2_VC_NO	Cystophora cristata	adult	visual cortex	normoxia	2
SA236984	Ccr3-3_VC_NO	Cystophora cristata	adult	visual cortex	normoxia	3
SA236985	Ccr4-3_VC_NO	Cystophora cristata	adult	visual cortex	normoxia	3
SA236986	Ccr1-3_VC_NO	Cystophora cristata	adult	visual cortex	normoxia	3
SA236987	Ccr2-3_VC_NO	Cystophora cristata	adult	visual cortex	normoxia	3
SA236988	Ccr4-1_VC_HONO	Cystophora cristata	adult	visual cortex	reoxygenation	1
SA236989	Ccr3-1_VC_HONO	Cystophora cristata	adult	visual cortex	reoxygenation	1
SA236990	Ccr1-1_VC_HONO	Cystophora cristata	adult	visual cortex	reoxygenation	1
SA236991	Ccr2-1_VC_HONO	Cystophora cristata	adult	visual cortex	reoxygenation	1
SA236992	Ccr2-2_VC_HONO	Cystophora cristata	adult	visual cortex	reoxygenation	2
SA236993	Ccr1-2_VC_HONO	Cystophora cristata	adult	visual cortex	reoxygenation	2
SA236994	Ccr3-2_VC_HONO	Cystophora cristata	adult	visual cortex	reoxygenation	2
SA236995	Ccr4-2_VC_HONO	Cystophora cristata	adult	visual cortex	reoxygenation	2
SA236996	Ccr4-3_VC_HONO	Cystophora cristata	adult	visual cortex	reoxygenation	3
SA236997	Ccr3-3_VC_HONO	Cystophora cristata	adult	visual cortex	reoxygenation	3
SA236998	Ccr2-3_VC_HONO	Cystophora cristata	adult	visual cortex	reoxygenation	3
SA236999	Ccr1-3_VC_HONO	Cystophora cristata	adult	visual cortex	reoxygenation	3

Showing results 1 to 36 of 36

Showing results 1 to 36 of 36

Collection:

Collection ID:	CO002441
Collection Summary:	Hooded seals (Cystophora cristata) were captured in the pack ice of the Greenland Sea under permits from relevant Norwegian and Greenland authorities. The adult hooded seals were euthanized immediately following capture, by sedation with intramuscular injection of zolazepam/tiletamine (1.5–2.0 mg per kg of body mass), followed by catheterization of the extradural intravertebral vein and i.v. injection of an overdose of pentobarbital (Euthasol vet., Le Vet B.V., Netherlands; 30 mg per kg of body mass). All animal handling was in accordance with the Norwegian Animal Welfare Act and with approvals from the National Animal Research Authority of Norway (permits no. 7247, 19305 and 22751). Fresh visual cortex samples from hooded seal adults were minced and placed in cooled (4 °C) artificial cerebrospinal fluid (aCSF; 128 mM NaCl, 3 mM KCl, 1.5 mM CaCl2, 1 mM MgCl2, 24 mM NaHCO3, 0.5 mM NaH2PO4, 20 mM sucrose, 10 mM D-glucose) saturated with 95% O2−5% CO2 (normoxia) and further processed in vitro.
Sample Type:	Brain
Storage Conditions:	-80℃

Treatment:

Treatment ID:	TR002460
Treatment Summary:	Samples in aCSF were adjusted to 34±0.5°C for at least 20 min. Hypoxia was introduced and maintained for 60 min after switching the gas supply to 95% N2 and 5% CO2, to mimic the diving brain. To simulate conditions when the seal surfaces after a dive, samples were exposed to hypoxia followed by 20 min return to normoxia. After treatment, hypoxia and reoxygenation samples were immediately frozen in liquid nitrogen. Samples that were kept under normoxia in aCSF for 80 min were used as controls. All samples were transferred to and stored at -80°C until later use.

Treatment ID:

TR002460

Treatment Summary:

Samples in aCSF were adjusted to 34±0.5°C for at least 20 min. Hypoxia was introduced and maintained for 60 min after switching the gas supply to 95% N2 and 5% CO2, to mimic the diving brain. To simulate conditions when the seal surfaces after a dive, samples were exposed to hypoxia followed by 20 min return to normoxia. After treatment, hypoxia and reoxygenation samples were immediately frozen in liquid nitrogen. Samples that were kept under normoxia in aCSF for 80 min were used as controls. All samples were transferred to and stored at -80°C until later use.

Sample Preparation:

Sampleprep ID:	SP002454
Sampleprep Summary:	The extraction protocol was performed slightly modified according to the method of Bligh and Dyer (Bligh and Dyer 1959). About 20 mg sample was weighed into a 2.0 ml reaction tube (Eppendorf, Hamburg, Germany). Two steel balls (3.6 mm), 100 µl chloroform and 200 µl methanol were added to the sample. The mixture was homogenized in a ball mill (1 min, 3.1 m/s Bead Ruptor 24, Omni International IM, GA, USA)). Afterwards 200 µl water and 100 µl chloroform were added and again processed in the ball mill (1 min, 3.1 m/s). The homogenized sample was then centrifuged (20 min, 16.000xg, 5 °C, Sigma 3-16PK, Sigma, Osterode, Germany). A quality control sample (QC) was prepared by transferring 30 µl of each sample into a new vial. The organic chloroform phase was directly used for measurement. Because of limited sample number, technical triplicates of each sample were measured.

Sampleprep ID:

SP002454

Sampleprep Summary:

The extraction protocol was performed slightly modified according to the method of Bligh and Dyer (Bligh and Dyer 1959). About 20 mg sample was weighed into a 2.0 ml reaction tube (Eppendorf, Hamburg, Germany). Two steel balls (3.6 mm), 100 µl chloroform and 200 µl methanol were added to the sample. The mixture was homogenized in a ball mill (1 min, 3.1 m/s Bead Ruptor 24, Omni International IM, GA, USA)). Afterwards 200 µl water and 100 µl chloroform were added and again processed in the ball mill (1 min, 3.1 m/s). The homogenized sample was then centrifuged (20 min, 16.000xg, 5 °C, Sigma 3-16PK, Sigma, Osterode, Germany). A quality control sample (QC) was prepared by transferring 30 µl of each sample into a new vial. The organic chloroform phase was directly used for measurement. Because of limited sample number, technical triplicates of each sample were measured.

Combined analysis:

Analysis ID	AN003852	AN003853
Analysis type	MS	MS
Chromatography type	Reversed phase	Reversed phase
Chromatography system	Dionex Ultimate 3000 UPLC system (Dionex, Idstein, Germany)	Dionex Ultimate 3000 UPLC system (Dionex, Idstein, Germany)
Column	Phenomenex Kinetex C18 (150 x 2.1mm,1.7um)	Phenomenex Kinetex C18 (150 x 2.1mm,1.7um)
MS Type	ESI	ESI
MS instrument type	QTOF	QTOF
MS instrument name	Bruker Daltonics maXis 3G	Bruker Daltonics maXis 3G
Ion Mode	POSITIVE	NEGATIVE
Units	Peak Area	Peak Area

Chromatography:

Chromatography ID:	CH002851
Chromatography Summary:	LC experiments were carried out using a RP C-18 column (150 × 2.1 mm, 1.7 μm, Phenomenex, Aschaffenburg, Germany) together with a Dionex Ultimate 3000 UPLC system (Dionex, Idstein, Germany). The mobile phase consisted of water (solvent A) and mixture of acetonitrile and isopropanol (1:3, v/v) (solvent B). Both eluents contained 10 mMol/L ammonium formate for measurements in positive ionization mode and 0.02% acetic acid for measurements in negative ionization mode. The column oven was set at 50°C and the flow rate was 300 µL/min. The gradient elution was as follows: 55% B (0-2 minutes); 55% to 75% B (2-4 minutes); 75% to 100% B (4-18 minutes); 100% B (18-23 minutes), 55% B (23-24 minutes); 55% B (24-27 minutes). For measurements in positive ionization mode, 2 µL of the sample extracts were injected while for analyzes in negative ionization mode 8 µL were used. The samples were analyzed in randomized order, with one blank sample and one QC sample being measured after each of the five animal samples. The autosampler in which the samples were stored during the measurement was set to 4° C.
Instrument Name:	Dionex Ultimate 3000 UPLC system (Dionex, Idstein, Germany)
Column Name:	Phenomenex Kinetex C18 (150 x 2.1mm,1.7um)
Column Temperature:	50°C
Flow Gradient:	55% B (0-2 minutes); 55% to 75% B (2-4 minutes); 75% to 100% B (4-18 minutes); 100% B (18-23 minutes), 55% B (23-24 minutes); 55% B (24-27 minutes)
Flow Rate:	300 µL/min
Internal Standard:	10 mMol/L ammonium formate for measurements in positive ionization mode and 0.02% acetic acid for measurements in negative ionization mode
Sample Injection:	2 µL of sample extracts were injected for measurements in positive ionization mode and 2µl of the sample extracts were injected for analyzes in negative ionization mode
Solvent A:	100% water
Solvent B:	25% acetonitrile/75% isopropanol
Chromatography Type:	Reversed phase

MS:

MS ID:	MS003593
Analysis ID:	AN003852
Instrument Name:	Bruker Daltonics maXis 3G
Instrument Type:	QTOF
MS Type:	ESI
MS Comments:	The data were recorded at 1 Hz over a mass range of m/z 80-1100. Further parameters were: end plate offset -500 V, capillary -4500 V, nebulizer pressure 4.0 bar, dry gas 9.0 L/min at 200 °C dry temperature. At the beginning of the measurements, the mass spectrometer was calibrated using sodium formate clusters. At the end of each sample run, a further calibration was carried out using the cluster solutions. Acquired experimental mass spectra were recalibrated with Bruker Data Analysis Software 4.2 (Bruker Daltonics, Bremen, Germany) using the mentioned sodium formate clusters. Afterwards, data were exported to netCDF file format. Data preprocessing was performed with R package xcms 3.6.2 (Smith et al. 2006) in R version 3.6.3 (R Core Team 2021). Parameters for processing were optimized based on existing tools and scripts (Libiseller et al. 2015; Manier et al. 2019). After reading in recalibrated netCDF files, features were detected with findChromPeaks function and CentWaveParam (peakwidth = c(10, 40), ppm = 20, snthresh = 10, mzdiff = 0.015, prefilter = c(0, 0), noise = 0)). Retention time was corrected with adjustRtime function and ObiwarpParam (binSize = 1.0). Feature correspondence was achieved with groupChromPeaks function and PeakDensityParam (sampleGroups = xdata$sample_group, bw = 1) as well as missing value imputation with fillChromPeaks function with FillChromPeaksParam (fixedRt = ChromPeakwidth/2)). ChromPeakwidth was calculated as average peak width of detected chromatographic peaks. Adducts and isotopes of features were annotated using R package CAMERA 1.40.0 (Kuhl et al. 2012). Features in the QC samples with a relative standard deviation over 30%, blank intensity contribution over 10% and QC sample count below 60% were removed before further statistical analysis.
Ion Mode:	POSITIVE
Capillary Voltage:	-4500 V
Dry Gas Flow:	9.0 L/min
Dry Gas Temp:	200 °C
Nebulizer:	4.0 bar

MS ID:	MS003594
Analysis ID:	AN003853
Instrument Name:	Bruker Daltonics maXis 3G
Instrument Type:	QTOF
MS Type:	ESI
MS Comments:	The data were recorded at 1 Hz over a mass range of m/z 80-1100. Further parameters were: end plate offset -500 V, capillary +4500 V, nebulizer pressure 4.0 bar, dry gas 9.0 L/min at 200 °C dry temperature. At the beginning of the measurements, the mass spectrometer was calibrated using sodium acetate clusters. At the end of each sample run, a further calibration was carried out using the cluster solutions. Acquired experimental mass spectra were recalibrated with Bruker Data Analysis Software 4.2 (Bruker Daltonics, Bremen, Germany) using the mentioned sodium acetate clusters. Afterwards, data were exported to netCDF file format. Data preprocessing was performed with R package xcms 3.6.2 (Smith et al. 2006) in R version 3.6.3 (R Core Team 2021). Parameters for processing were optimized based on existing tools and scripts (Libiseller et al. 2015; Manier et al. 2019). After reading in recalibrated netCDF files, features were detected with findChromPeaks function and CentWaveParam (peakwidth = c(10, 40), ppm = 20, snthresh = 10, mzdiff = 0.015, prefilter = c(0, 0), noise = 0)). Retention time was corrected with adjustRtime function and ObiwarpParam (binSize = 1.0). Feature correspondence was achieved with groupChromPeaks function and PeakDensityParam (sampleGroups = xdata$sample_group, bw = 1) as well as missing value imputation with fillChromPeaks function with FillChromPeaksParam (fixedRt = ChromPeakwidth/2)). ChromPeakwidth was calculated as average peak width of detected chromatographic peaks. Adducts and isotopes of features were annotated using R package CAMERA 1.40.0 (Kuhl et al. 2012). Features in the QC samples with a relative standard deviation over 30%, blank intensity contribution over 10% and QC sample count below 60% were removed before further statistical analysis.
Ion Mode:	NEGATIVE
Capillary Voltage:	+4500 V
Dry Gas Flow:	9.0 L/min
Dry Gas Temp:	200 °C
Nebulizer:	4.0 bar