Summary of Study ST002055

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 PR001300. The data can be accessed directly via it's Project DOI: 10.21228/M8P69K This work is supported by NIH grant, U2C- DK119886.

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

Study ID	ST002055
Study Title	Metabolomic Profiling of Human Pluripotent Stem Cell Differentiation into Lung Progenitors
Study Summary	Metabolism is vital to cellular function and tissue homeostasis during human lung development. In utero, embryonic pluripotent stem cells undergo endodermal differentiation towards a lung progenitor cell fate that can be mimicked in vitro using induced human pluripotent stem cells (hiPSCs) to study genetic mutations. To identify differences between wild type and surfactant protein B (SFTPB)-deficient cell lines during endoderm specification towards lung, we used an untargeted metabolomics approach to evaluate the developmental changes in metabolites. We found that the metabolites most enriched during the differentiation from pluripotent stem cell to lung progenitor cell, regardless of cell line, were sphingomyelins and phosphatidylcholines, two important lipid classes in fetal lung development. The SFTPB mutation had no metabolic impact on early endodermal lung development. The identified metabolite signatures during lung progenitor cell differentiation may be utilized as biomarkers for normal embryonic lung development.
Institute	The Hospital for Sick Children
Last Name	Post
First Name	Martin
Address	555 University Avenue
Email	martin.post@sickkids.ca
Phone	4168136772
Submit Date	2021-06-29
Raw Data Available	Yes
Raw Data File Type(s)	wiff
Analysis Type Detail	LC-MS/MS(Dir. Inf.)
Release Date	2022-01-13
Release Version	1

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Project:

Project ID:	PR001300
Project DOI:	doi: 10.21228/M8P69K
Project Title:	Metabolomic Profiling of Human Pluripotent Stem Cell Differentiation into Lung Progenitors
Project Type:	Developmental metabolites and Biomarker discovery
Project Summary:	Metabolism is vital to cellular function and tissue homeostasis during human lung development. In utero, embryonic pluripotent stem cells undergo endodermal differentiation towards a lung progenitor cell fate that can be mimicked in vitro using induced human pluripotent stem cells (hiPSCs) to study genetic mutations. To identify differences between wild type and surfactant protein B (SFTPB)-deficient cell lines during endoderm specification towards lung, we used an untargeted metabolomics approach to evaluate the developmental changes in metabolites. We found that the metabolites most enriched during the differentiation from pluripotent stem cell to lung progenitor cell, regardless of cell line, were sphingomyelins and phosphatidylcholines, two important lipid classes in fetal lung development. The SFTPB mutation had no metabolic impact on early endodermal lung development. The identified metabolite signatures during lung progenitor cell differentiation may be utilized as biomarkers for normal embryonic lung development.
Institute:	The Hospital for Sick Children
Last Name:	Post
First Name:	Martin
Address:	555 University Avenue
Email:	martin.post@sickkids.ca
Phone:	4168136772

Subject:

Subject ID:	SU002137
Subject Type:	Cultured cells
Subject Species:	Homo sapiens
Taxonomy ID:	9606

Factors:

Subject type: Cultured cells; Subject species: Homo sapiens (Factor headings shown in green)

mb_sample_id	local_sample_id	Differentiation stage
SA193726	60 - ICE 12	Anterior Foregut Endoderm
SA193727	28 - NCRM1 12	Anterior Foregut Endoderm
SA193728	26 - NCRM1 10	Anterior Foregut Endoderm
SA193729	25 - NCRM1 9	Anterior Foregut Endoderm
SA193730	59 - ICE 11	Anterior Foregut Endoderm
SA193731	42 - ICD 10	Anterior Foregut Endoderm
SA193732	57 - ICE 9	Anterior Foregut Endoderm
SA193733	58 - ICE 10	Anterior Foregut Endoderm
SA193734	44 - ICD 12	Anterior Foregut Endoderm
SA193735	43 - ICD 11	Anterior Foregut Endoderm
SA193736	41 - ICD 9	Anterior Foregut Endoderm
SA193737	27 - NCRM1 11	Anterior Foregut Endoderm
SA193738	10 - CA1 10	Anterior Foregut Endoderm
SA193739	9 - CA1 9	Anterior Foregut Endoderm
SA193740	11 - CA1 11	Anterior Foregut Endoderm
SA193741	12 - CA1 12	Anterior Foregut Endoderm
SA193742	7 - CA1 7	Definitive Endoderm
SA193743	56 - ICE 8	Definitive Endoderm
SA193744	6 - CA1 6	Definitive Endoderm
SA193745	40 - ICD 8	Definitive Endoderm
SA193746	39 - ICD 7	Definitive Endoderm
SA193747	37 - ICD 5	Definitive Endoderm
SA193748	8 - CA1 8	Definitive Endoderm
SA193749	55 - ICE 7	Definitive Endoderm
SA193750	5 - CA1 5	Definitive Endoderm
SA193751	54 - ICE 6	Definitive Endoderm
SA193752	22 - NCRM1 6	Definitive Endoderm
SA193753	21 - NCRM1 5	Definitive Endoderm
SA193754	53 - ICE 5	Definitive Endoderm
SA193755	23 - NCRM1 7	Definitive Endoderm
SA193756	24 - NCRM1 8	Definitive Endoderm
SA193757	38 - ICD 6	Definitive Endoderm
SA193778	33 - ICD 1	iPSC
SA193779	20 - NCRM1 4	iPSC
SA193780	19 - NCRM1 3	iPSC
SA193781	18 - NCRM1 2	iPSC
SA193782	17 - NCRM1 1	iPSC
SA193783	34 - ICD 2	iPSC
SA193784	35 - ICD 3	iPSC
SA193785	51 - ICE 3	iPSC
SA193786	50 - ICE 2	iPSC
SA193787	49 - ICE 1	iPSC
SA193788	36 - ICD 4	iPSC
SA193789	52 - ICE 4	iPSC
SA193758	45 - ICD 13	Lung Progenitor Cell
SA193759	46 - ICD 14	Lung Progenitor Cell
SA193760	47 - ICD 15	Lung Progenitor Cell
SA193761	48 - ICD 16	Lung Progenitor Cell
SA193762	31 - NCRM1 15	Lung Progenitor Cell
SA193763	64 - ICE 16	Lung Progenitor Cell
SA193764	13 - CA1 13	Lung Progenitor Cell
SA193765	16 - CA1 16	Lung Progenitor Cell
SA193766	15 - CA1 15	Lung Progenitor Cell
SA193767	63 - ICE 15	Lung Progenitor Cell
SA193768	62 - ICE 14	Lung Progenitor Cell
SA193769	14 - CA1 14	Lung Progenitor Cell
SA193770	32 - NCRM1 16	Lung Progenitor Cell
SA193771	30 - NCRM1 14	Lung Progenitor Cell
SA193772	29 - NCRM1 13	Lung Progenitor Cell
SA193773	61 - ICE 13	Lung Progenitor Cell
SA193774	1 - CA1 1	PSC
SA193775	4 - CA1 4	PSC
SA193776	3 - CA1 3	PSC
SA193777	2 - CA1 2	PSC

Showing results 1 to 64 of 64

Showing results 1 to 64 of 64

Collection:

Collection ID:	CO002130
Collection Summary:	Samples were analyzed for 180 metabolites using the AbsoluteIDQ® p180 kit from Biocrates Life Sciences AG at the Analytical Facility for Bioactive Molecules (The Hospital for Sick Children, Toronto, Canada). Collected cell pellets were resuspended in 15 % ice-cold 10 mM Phosphate Buffer (PB) + 85 % EtOH as per AbsoluteIDQ® p180 kit protocol. Resuspended cells were subjected to three rounds of sonication and rapid freeze thawing. Final suspension was then centrifuged at 20,000 x g for 10 minutes at 4°C. A small aliquot was taken for protein assay, and the remainder of the supernatant was used for metabolic analysis. Samples, standards, and controls (10 mL each) were added to the Biocrates 96-well filter plate with internal standard, dried under nitrogen, derivatized with phenyl isothiocyanate, and then extracted with methanol, as per kit instructions.
Sample Type:	human cells

Treatment:

Treatment ID:	TR002149
Treatment Summary:	No treatment

Sample Preparation:

Sampleprep ID:	SP002143
Sampleprep Summary:	At each differentiation step, DE, AFE and LPC, cells were analyzed by FACS for stage specific markers. The differentiated cells were harvested with TrypLE at 37 °C for 5-10 minutes and collected by centrifugation at 300 g for 5 minutes at room temperature. The cell pellets were resuspended in 3% (v/v) FBS in PBS, cell aggregates were removed using a cell strainer with a 40-µm pore size and single cells were collected. For surface antigens, the cells were incubated with primary antibodies for 30 minutes on ice with gentle shaking, washed twice with 3% (v/v) FBS in PBS, and if necessary, incubated with the secondary antibodies for 30 minutes followed by two more rinses with 3% (v/v) FBS in PBS. For DE cells, we used PE conjugated mouse anti-human CXCR4 and APC conjugated mouse anti-human cKit antibodies; AFE cells were stained with PE-conjugated mouse anti-human CD56 and APC conjugated mouse anti-human CD271 antibodies and LPCs we identified using mouse anti-human CPM antibody. Alexa Fluor 488 donkey anti-mouse IgG was used as the secondary antibody against primary CPM antibody. The cells were either sorted using the BD aria FACS sorter at the Sick Kids FACS core and/or analyzed using a Beckman Coulter Gallios flow cytometer. Unstained controls were used to set up gates for FSC and SSC and double stained cells underwent fluorescence minus one (FMO) to ensure accurate gating. Sorted cells were collected and the spun down into a cell pellet and stored in -80C degrees for further processing. The endodermal differentiations and cell sorts were repeated at four different times with two biological repeats.

Sampleprep ID:

SP002143

Sampleprep Summary:

At each differentiation step, DE, AFE and LPC, cells were analyzed by FACS for stage specific markers. The differentiated cells were harvested with TrypLE at 37 °C for 5-10 minutes and collected by centrifugation at 300 g for 5 minutes at room temperature. The cell pellets were resuspended in 3% (v/v) FBS in PBS, cell aggregates were removed using a cell strainer with a 40-µm pore size and single cells were collected. For surface antigens, the cells were incubated with primary antibodies for 30 minutes on ice with gentle shaking, washed twice with 3% (v/v) FBS in PBS, and if necessary, incubated with the secondary antibodies for 30 minutes followed by two more rinses with 3% (v/v) FBS in PBS. For DE cells, we used PE conjugated mouse anti-human CXCR4 and APC conjugated mouse anti-human cKit antibodies; AFE cells were stained with PE-conjugated mouse anti-human CD56 and APC conjugated mouse anti-human CD271 antibodies and LPCs we identified using mouse anti-human CPM antibody. Alexa Fluor 488 donkey anti-mouse IgG was used as the secondary antibody against primary CPM antibody. The cells were either sorted using the BD aria FACS sorter at the Sick Kids FACS core and/or analyzed using a Beckman Coulter Gallios flow cytometer. Unstained controls were used to set up gates for FSC and SSC and double stained cells underwent fluorescence minus one (FMO) to ensure accurate gating. Sorted cells were collected and the spun down into a cell pellet and stored in -80C degrees for further processing. The endodermal differentiations and cell sorts were repeated at four different times with two biological repeats.

Combined analysis:

Analysis ID	AN003346	AN003347
Analysis type	MS	MS
Chromatography type	Reversed phase	None (Direct infusion)
Chromatography system	Agilent 1290 Infinity	-
Column	Agilent Eclipse XDB-C18 (100 x 3.0mm)	-
MS Type	ESI	ESI
MS instrument type	Triple quadrupole	Triple quadrupole
MS instrument name	ABI Sciex 5500 QTrap	ABI Sciex 5500 QTrap
Ion Mode	POSITIVE	UNSPECIFIED
Units	uM	uM

Chromatography:

Chromatography ID:	CH002477
Instrument Name:	Agilent 1290 Infinity
Column Name:	Agilent Eclipse XDB-C18 (100 x 3.0mm)
Chromatography Type:	Reversed phase

Chromatography ID:	CH002478
Instrument Name:	-
Column Name:	-
Chromatography Type:	None (Direct infusion)

MS:

MS ID:	MS003115
Analysis ID:	AN003346
Instrument Name:	ABI Sciex 5500 QTrap
Instrument Type:	Triple quadrupole
MS Type:	ESI
MS Comments:	Analyst1.7 (Sciex); MetIDQ (Biocrates)
Ion Mode:	POSITIVE

MS ID:	MS003116
Analysis ID:	AN003347
Instrument Name:	ABI Sciex 5500 QTrap
Instrument Type:	Triple quadrupole
MS Type:	ESI
MS Comments:	Analyst1.7 (Sciex); MetIDQ (Biocrates)
Ion Mode:	UNSPECIFIED