Summary of Study ST002396

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 PR001543. The data can be accessed directly via it's Project DOI: 10.21228/M87T4V 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	ST002396
Study Title	p53 K316P mutation results in increased liver triglyceride levels and increased rates of de novo lipogenesis.
Study Summary	Our lab generated the p53 K316P mouse, which mimicks a common amino acid change found in bats. The K316P mutation, found in the nuclear localization signal of p53, results in increased cytoplasmic localization of p53. We found that K316P mutant mice develop several metabolic phenotypes, including increased body fat percentage, and increased liver lipid levels. In order to determine the mechanism through which K316P mutation increases liver lipid levels, we performed metabolomic analysis of mouse livers from WT and K316P mutant mice. Mouse livers were isolated from four wild type (WT) and four p53 K316P (M) mice for lipidomic analysis. Samples were isolated and flash frozen in liquid nitrogen. Lipids were then extracted from each liver sample and analyzed using mass spectrometry.
Institute	University of North Carolina
Last Name	Sanford
First Name	Jack
Address	450 West Drive, Chapel Hill, NC, 27514
Email	jsan4d@email.unc.edu
Phone	3019284726
Submit Date	2022-12-07
Raw Data Available	Yes
Raw Data File Type(s)	mzXML
Analysis Type Detail	LC-MS
Release Date	2022-12-27
Release Version	1

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Project:

Project ID:	PR001543
Project DOI:	doi: 10.21228/M87T4V
Project Title:	p53 K316P mouse liver lipidomics analysis
Project Summary:	Mouse livers were isolated from four wild type (WT) and four p53 K316P (M) mice for lipidomic analysis. Samples were isolated and flash frozen in liquid nitrogen. Lipids were then extracted from each liver sample and analyzed using mass spectrometry.
Institute:	University of North Carolina
Last Name:	Sanford
First Name:	Jack
Address:	450 West Drive, Chapel Hill, NC, 27514
Email:	jsan4d@email.unc.edu
Phone:	3019284726

Subject:

Subject ID:	SU002485
Subject Type:	Mammal
Subject Species:	Mus musculus
Taxonomy ID:	10090

Factors:

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

mb_sample_id	local_sample_id	experimental factor(s)
SA239023	WT-22R	p53 +/+
SA239024	WT-24R	p53 +/+
SA239025	WT-21RL	p53 +/+
SA239026	WT-8RL	p53 +/+
SA239027	m-6R	p53 K316P m/m
SA239028	m-12L	p53 K316P m/m
SA239029	m-41RL	p53 K316P m/m
SA239030	m-6L	p53 K316P m/m

Showing results 1 to 8 of 8

Showing results 1 to 8 of 8

Collection:

Collection ID:	CO002478
Collection Summary:	Mouse liver samples were collected from mice and immediately flash frozen in liquid nitrogen. Frozen tissue samples were crushed using a morter and pestle on dry ice to homogenize tissue prior to lipid extraction.
Sample Type:	Liver

Treatment:

Treatment ID:	TR002497
Treatment Summary:	Male mice were C57BL/6J background, kept on a 12hr day/night cycle. Mice were 3-4 months old at the time of tissue isolation. Four littermate pairs were analyzed.

Sample Preparation:

Sampleprep ID:	SP002491
Sampleprep Summary:	Mouse liver sections were weighed into Eppendorf tubes. The liver tissue was then mashed with a spatula prior to extraction. The samples were extracted using a liquid liquid partition with water (250 µL), methanol (300 µL), and MTBE (1 mL). Avanti’s deuterated lipid mix, Equisplash, was used as an internal standard. This was spiked into the methanol at 1.5 µg/mL and used for extraction. The extracts were centrifuged at 20,000 rcf for 10 min. The top layer was removed, dried down, and reconstituted in 1 mL of IPA for analysis.

Sampleprep ID:

SP002491

Sampleprep Summary:

Mouse liver sections were weighed into Eppendorf tubes. The liver tissue was then mashed with a spatula prior to extraction. The samples were extracted using a liquid liquid partition with water (250 µL), methanol (300 µL), and MTBE (1 mL). Avanti’s deuterated lipid mix, Equisplash, was used as an internal standard. This was spiked into the methanol at 1.5 µg/mL and used for extraction. The extracts were centrifuged at 20,000 rcf for 10 min. The top layer was removed, dried down, and reconstituted in 1 mL of IPA for analysis.

Combined analysis:

Analysis ID	AN003903
Analysis type	MS
Chromatography type	Reversed phase
Chromatography system	Waters Acquity H-Class
Column	Waters Acquity BEH C18 (100 x 2.1mm,1.7um)
MS Type	ESI
MS instrument type	Orbitrap
MS instrument name	Thermo Q Exactive HF-X Orbitrap
Ion Mode	UNSPECIFIED
Units	peak area

Chromatography:

Chromatography ID:	CH002889
Chromatography Summary:	Analysis was performed using a Thermo Q Exactive Plus coupled to a Waters Acquity H-Class LC. A 100 mm x 2.1 mm, 1.7 µm Waters BEH C18 column was used for separations. The following mobile phases were used: A- 60/40 ACN/H20 B- 90/10 IPA/ACN; both mobile phases had 10 mM Ammonium Formate and 0.1% Formic Acid. A flow rate of 0.2 mL/min was used. Starting composition was 32% B, which increased to 40% B at 1 min (held until 1.5 min) then 45% B at 4 minutes. This was increased to 50% B at 5 min, 60% B at 8 min, 70% B at 11 min, and 80% B at 14 min (held until 16 min). At 16 min the composition switched back to starting conditions (32% B) and was held for 4 min to re-equilibrate the column. Samples were analyzed in positive/negative switching ionization mode with top 5 data dependent fragmentation.
Methods Filename:	Sanford_2022_Lipidomics_protocol.docx
Instrument Name:	Waters Acquity H-Class
Column Name:	Waters Acquity BEH C18 (100 x 2.1mm,1.7um)
Chromatography Type:	Reversed phase

MS:

MS ID:	MS003642
Analysis ID:	AN003903
Instrument Name:	Thermo Q Exactive HF-X Orbitrap
Instrument Type:	Orbitrap
MS Type:	ESI
MS Comments:	Analysis was performed using a Thermo Q Exactive Plus coupled to a Waters Acquity H-Class LC. A 100 mm x 2.1 mm, 2.1 µm Waters BEH C18 column was used for separations. The following mobile phases were used: A- 60/40 ACN/H20 B- 90/10 IPA/ACN; both mobile phases had 10 mM Ammonium Formate and 0.1% Formic Acid. A flow rate of 0.2 mL/min was used. Starting composition was 32% B, which increased to 40% B at 1 min (held until 1.5 min) then 45% B at 4 minutes. This was increased to 50% B at 5 min, 60% B at 8 min, 70% B at 11 min, and 80% B at 14 min (held until 16 min). At 16 min the composition switched back to starting conditions (32% B) and was held for 4 min to re-equilibrate the column. Samples were analyzed in positive/negative switching ionization mode with top 5 data dependent fragmentation.
Ion Mode:	UNSPECIFIED
Analysis Protocol File:	Sanford_2022_Lipidomics_protocol.docx