Summary of Study ST002781

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 PR001715. The data can be accessed directly via it's Project DOI: 10.21228/M81D9R This work is supported by NIH grant, U2C- DK119886.

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

Perform statistical analysis | Show all samples | Show named metabolites | Download named metabolite data
Download mwTab file (text) | Download mwTab file(JSON)

Study ID	ST002781
Study Title	Lipidomics analysis of maternal obesity model - wild type
Study Summary	10μl liver tissue of 11-12 weeks old male mice from various diet groups with various genetic background were homogenized and lipids were extracted for shotgun lipidomics experiments. Raw files were converted to .mzml files and imported into and analyzed by LipidXplorer software using custom mfql files to identify sample lipids and internal standards. For further data processing, absolute amounts were calculated using the internal standard intensities followed by the calculated mol% of the identified lipids. For wild-type C57BL/6JRcc mice, diet groups are CDm CDl CD, CDm CDl HFD, CDm HFDl HFD, HFDm CDl CD, HFDm CDl HFD, HFDm HFDl CD and HFDm CDl CD. m: maternal diet, l: lactation phase diet.
Institute	University of Bonn
Department	LIMES
Laboratory	Mass Lab
Last Name	Mass
First Name	Elvira
Address	Carl-Troll-Str. 31, 53115 Bonn, Germany
Email	elvira.mass@uni-bonn.de
Phone	+49 0228 / 73 6 28 48
Submit Date	2023-07-02
Num Groups	6
Total Subjects	28
Analysis Type Detail	MS(Dir. Inf.)
Release Date	2023-08-01
Release Version	1

Select appropriate tab below to view additional metadata details:

Project:

Project ID:	PR001715
Project DOI:	doi: 10.21228/M81D9R
Project Title:	Developmental programming of Kupffer cells by maternal obesity causes fatty liver disease in the offspring
Project Summary:	Kupffer cells (KCs) are tissue-resident macrophages which colonize the developing liver early during embryogenesis. Throughout development and adulthood, KCs have distinct core functions that are essential for liver and organismal homeostasis, such as supporting fetal erythropoiesis as well as postnatal erythrocyte recycling and liver metabolism. KCs acquire their tissue-specific transcriptional signature immediately after colonizing the liver, mature together with the tissue, and adapt to the tissue’s function. However, whether perturbation of macrophage core functions during development may contribute to or cause disease at postnatal stages is poorly understood. Here, we utilize a maternal obesity model to disturb KC functions during gestation. We show that offspring born to obese mothers develop fatty liver disease that is accompanied by a local pro-inflammatory response, a phenotype that is augmented if the offspring is kept on control diet after birth. Further, transcriptional analyses reveal that KCs undergo developmental programming through the maternal high-fat diet, which lasts until adulthood. The offspring’s KC developmental programming is irreversible despite the switch to control diet and leads to increased lipid uptake in hepatocytes mediated via paracrine factors stemming from KCs. The transcriptional programming of KCs and the fatty liver disease phenotype are rescued by genetic depletion of hypoxia-inducible factor alpha (Hif-1alpha) in macrophages during gestation. These results demonstrate that macrophages rely on an undisturbed development to fulfil their core functions and support organ homeostasis during adulthood, and establish developmental programming of KCs as a therapeutic strategy for metabolic disorders, such as fatty liver disease.
Institute:	University of Bonn
Department:	LIMES
Laboratory:	Mass Lab
Last Name:	Mass
First Name:	Elvira
Address:	Carl-Troll-Str. 31, 53115 Bonn, Germany
Email:	elvira.mass@uni-bonn.de
Phone:	+49 0228 / 73 6 28 48
Funding Source:	DFG
Publications:	in preparation
Contributors:	Nora Balzer, Iva Splichalova, Hao Huang, Stephan Grein, Lea Seep

Subject:

Subject ID:	SU002888
Subject Type:	Mammal
Subject Species:	Mus musculus
Taxonomy ID:	10090
Genotype Strain:	C57BL/6JRcc
Age Or Age Range:	10-12 weeks
Animal Housing:	specific pathogen-free conditions
Animal Light Cycle:	12-h light/dark cycle

Factors:

Subject type: Mammal; Subject species: Mus musculus (Factor headings shown in green)

mb_sample_id	local_sample_id	diet
SA298596	CD_CD_CD_103	CD_CD_CD
SA298597	CD_CD_CD_106	CD_CD_CD
SA298598	CD_CD_CD_105	CD_CD_CD
SA298599	CD_CD_HFD_207	CD_CD_HFD
SA298600	CD_CD_HFD_205	CD_CD_HFD
SA298601	CD_CD_HFD_206	CD_CD_HFD
SA298602	CD_CD_HFD_201	CD_CD_HFD
SA298603	CD_CD_HFD_200	CD_CD_HFD
SA298604	CD_CD_HFD_203	CD_CD_HFD
SA298605	HFD_CD_CD_803	HFD_CD_CD
SA298606	HFD_CD_CD_801	HFD_CD_CD
SA298607	HFD_CD_CD_802	HFD_CD_CD
SA298608	HFD_CD_CD_800	HFD_CD_CD
SA298609	HFD_CD_HFD_703	HFD_CD_HFD
SA298610	HFD_CD_HFD_701	HFD_CD_HFD
SA298611	HFD_CD_HFD_702	HFD_CD_HFD
SA298612	HFD_CD_HFD_700	HFD_CD_HFD
SA298613	HFD_HFD_CD_605	HFD_HFD_CD
SA298614	HFD_HFD_CD_604	HFD_HFD_CD
SA298615	HFD_HFD_CD_606	HFD_HFD_CD
SA298616	HFD_HFD_CD_603	HFD_HFD_CD
SA298617	HFD_HFD_CD_601	HFD_HFD_CD
SA298618	HFD_HFD_CD_602	HFD_HFD_CD
SA298619	HFD_HFD_HFD_504	HFD_HFD_HFD
SA298620	HFD_HFD_HFD_503	HFD_HFD_HFD
SA298621	HFD_HFD_HFD_501	HFD_HFD_HFD
SA298622	HFD_HFD_HFD_500	HFD_HFD_HFD
SA298623	HFD_HFD_HFD_502	HFD_HFD_HFD

Showing results 1 to 28 of 28

Showing results 1 to 28 of 28

Collection:

Collection ID:	CO002881
Collection Summary:	Livers were isolated from PBS-perfused mice, and 10 µg was homogenized in ddH2O using a Precellys homogenizer (Peqlab Biotechnology). The mice were subjected different diet schemes.
Collection Protocol Filename:	Lipidomics_Notes.pdf
Sample Type:	Liver

Treatment:

Treatment ID:	TR002897
Treatment Summary:	Samples were taken from the developed Maternal Obesity model. This model was generated as described in the Material and Methods section. No additional treatment was done.

Sample Preparation:

Sampleprep ID:	SP002894
Sampleprep Summary:	In this experiment, mouse livers were isolated and processed to extract lipids for analysis. The livers were homogenized and subjected to a series of centrifugation and phase separation steps to obtain the lipid samples. The extracted lipids were then prepared for further analysis by adding specific internal standards and a spray buffer, allowing for subsequent characterization and investigation.
Sampleprep Protocol Filename:	Lipidomics_Notes.pdf

Combined analysis:

Analysis ID	AN004528
Analysis type	MS
Chromatography type	None (Direct infusion)
Chromatography system	Thermo Q Exactive Plus
Column	none
MS Type	ESI
MS instrument type	Orbitrap
MS instrument name	Thermo Q Exactive Plus Orbitrap
Ion Mode	POSITIVE
Units	pmol/mg

Chromatography:

Chromatography ID:	CH003401
Instrument Name:	Thermo Q Exactive Plus
Column Name:	none
Column Temperature:	none
Flow Gradient:	-
Flow Rate:	10 µl/min
Injection Temperature:	260
Solvent A:	8/5/1 isopropanol/methanol/water; 10 mM ammonium acetate
Solvent B:	-
Chromatography Type:	None (Direct infusion)

MS:

MS ID:	MS004275
Analysis ID:	AN004528
Instrument Name:	Thermo Q Exactive Plus Orbitrap
Instrument Type:	Orbitrap
MS Type:	ESI
MS Comments:	Thermo Q Exactive Plus spectrometer equipped with the HESI II ion source. MS1 spectra (resolution 280 000) were recorded in 100 m/z windows from 250 to 1200 m/z (pos.) and 200 - 1700 m/z (neg.) followed by recording MS/MS spectra (res. 70 000) by data-independent acquisition in 1 m/z windows from 200 to 1200 (pos.) and 200 to 1700 (neg.) m/z. Raw files were converted to .mzml files and imported into and analyzed by LipidXplorer software using custom mfql files to identify sample lipids and internal standards. For further data processing, absolute amounts were calculated using the internal standard intensities followed by the calculated mol% of the identified lipids.
Ion Mode:	POSITIVE
Analysis Protocol File:	Lipidomics_Notes.pdf