Summary of Study ST003262

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 PR002024. The data can be accessed directly via it's Project DOI: 10.21228/M80C0P 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.

Study ID	ST003262
Study Title	A Covalent Creatine Kinase Inhibitor Ablates Glioblastoma Migration and Sensitizes Tumors to Oxidative Stress.
Study Type	Cki treatment on glioblastoma
Study Summary	Glioblastoma is a Grade 4 primary brain tumor defined by therapy resistance, diffuse infiltration, and near-uniform lethality. The underlying mechanisms are unknown, and no treatment has been curative. Using a recently developed kinase inhibitor (CKi), we explored the role of this inhibitor on GBM biology in vitro. While CKi minimally impacted GBM cell proliferation and viability, it significantly affected migration. In established GBM cell lines and patient-derived xenografts, CKi ablated both the migration and invasion of GBM cells. CKi also hindered radiation-induced migration. RNA-seq revealed a decrease in invasion-related genes, with an unexpected increase in glutathione metabolism and ferroptosis protection genes post-CKi treatment. The effects of CKi could be reversed by the addition of cell-permeable glutathione. Carbon-13 metabolite tracing indicated heightened glutathione biosynthesis post-CKi treatment. Combinatorial CKi blockade and glutathione inhibition or ferroptosis activation abrogated cell survival. Our data demonstrated that CKi perturbs promigratory and anti-ferroptotic roles in GBM, identifying the creatine kinase axis as a druggable target for GBM treatment.
Institute	Northwestern University, Feinberg School of Medicine
Department	Neurological Surgery
Laboratory	Jason Miska
Last Name	Miska
First Name	Jason
Address	676 N St. Clair
Email	jason.miska@northwestern.edu
Phone	8478678201
Submit Date	2024-06-14
Num Groups	2
Total Subjects	12
Raw Data Available	Yes
Raw Data File Type(s)	raw(Thermo)
Analysis Type Detail	LC-MS
Release Date	2024-06-18
Release Version	1

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Project:

Project ID:	PR002024
Project DOI:	doi: 10.21228/M80C0P
Project Title:	A Covalent Creatine Kinase Inhibitor Ablates Glioblastoma Migration and Sensitizes Tumors to Oxidative Stress
Project Type:	LC-MS/MS
Project Summary:	Glioblastoma is a Grade 4 primary brain tumor defined by therapy resistance, diffuse infiltration, and near-uniform lethality. The underlying mechanisms are unknown, and no treatment has been curative. Using a recently developed kinase inhibitor (CKi), we explored the role of this inhibitor on GBM biology in vitro. While CKi minimally impacted GBM cell proliferation and viability, it significantly affected migration. In established GBM cell lines and patient-derived xenografts, CKi ablated both the migration and invasion of GBM cells. CKi also hindered radiation-induced migration. RNA-seq revealed a decrease in invasion-related genes, with an unexpected increase in glutathione metabolism and ferroptosis protection genes post-CKi treatment. The effects of CKi could be reversed by the addition of cell-permeable glutathione. Carbon-13 metabolite tracing indicated heightened glutathione biosynthesis post-CKi treatment. Combinatorial CKi blockade and glutathione inhibition or ferroptosis activation abrogated cell survival. Our data demonstrated that CKi perturbs promigratory and anti-ferroptotic roles in GBM, identifying the creatine kinase axis as a druggable target for GBM treatment.
Institute:	Northwestern University, Feinberg School of Medicine
Department:	Neurological Surgery
Laboratory:	Jason Miska
Last Name:	Miska
First Name:	Jason
Address:	676 N St. Clair
Email:	jason.miska@northwestern.edu
Phone:	8478678201

Subject:

Subject ID:	SU003382
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	Sample source	Treatment
SA354220	Les-Jas-20230207-04	Brain	1hr
SA354221	Les-Jas-20230207-05	Brain	1hr
SA354222	Les-Jas-20230207-06	Brain	1hr
SA354223	Les-Jas-20230207-07	Brain	4hrs
SA354224	Les-Jas-20230207-08	Brain	4hrs
SA354225	Les-Jas-20230207-09	Brain	4hrs
SA354226	Les-Jas-20230207-10	Brain	8hrs
SA354227	Les-Jas-20230207-11	Brain	8hrs
SA354228	Les-Jas-20230207-12	Brain	8hrs
SA354229	Les-Jas-20230207-01	Brain	CTL
SA354230	Les-Jas-20230207-02	Brain	CTL
SA354231	Les-Jas-20230207-03	Brain	CTL

Showing results 1 to 12 of 12

Showing results 1 to 12 of 12

Collection:

Collection ID:	CO003375
Collection Summary:	GBM cells were cultured under the conditions indicated in the manuscript, then metabolites were collected using 80% methanol extraction.
Sample Type:	Brain

Treatment:

Treatment ID:	TR003391
Treatment Summary:	metabolites isolated from Cki treated cells. Samples 1-3 are control treatment, Sample 4-6 are 1 hour CKi treatment, Samples 7-9 are 4 hours CKi treatmet, and 10-12 are 8 hours CKi treatment.

Sample Preparation:

Sampleprep ID:	SP003389
Sampleprep Summary:	Isolated samples were dried using a SpeedVac. Acetonitrile (50%) was added to the tube for reconstitution following overtaxing for 30s. Sample solution was then centrifuged for 15min at 20,000g and 4°C. Supernatant was collected for LC-MS analysis.

Combined analysis:

Analysis ID	AN005346
Analysis type	MS
Chromatography type	HILIC
Chromatography system	Thermo Dionex Ultimate 3000
Column	Water's Xbridge amide (100 x 3mm, 3.5 um)
MS Type	ESI
MS instrument type	Orbitrap
MS instrument name	Thermo Q Exactive Plus Orbitrap
Ion Mode	UNSPECIFIED
Units	Peak area

Chromatography:

Chromatography ID:	CH004048
Chromatography Summary:	Samples were analyzed by high-performance LC (HPLC) and high-resolution MS and MS/MS (HPLC-MS/MS). The system consists of Thermo Q Exactive with an electrospray source and an UltiMate3000 (Thermo Fisher Scientific) series HPLC consisting of a binary pump, degasser, and autosampler outfitted with an XBridge Amide column (Waters; dimensions of 4.6 mm by 100 mm and a 3.5-μm particle size). The mobile phase A contained 95% water/5% acetonitrile (v/v), 20 mM ammonium hydroxide, and 20 mM ammonium acetate (pH 9.0); phase B was 100% acetonitrile. The gradient was performed as follows: 0 min, 15% A; 2.5 min, 30% A; 7 min, 43% A; 16 min, 62% A; 16.1 to 18 min, 75% A; and 18 to 25 min, 15% A with a flow rate of 400 µl/min.
Instrument Name:	Thermo Dionex Ultimate 3000
Column Name:	Water's Xbridge amide (100 x 3mm, 3.5 um)
Column Temperature:	-
Flow Gradient:	0 min, 15% A; 2.5 min, 30% A; 7 min, 43% A; 16 min, 62% A; 16.1 to 18 min, 75% A; and 18 to 25 min, 15% A
Flow Rate:	400 μl/min
Solvent A:	95% water/5% acetonitrile; 20 mM ammonium hydroxide; 20 mM ammonium acetate (pH 9.0)
Solvent B:	100% acetonitrile
Chromatography Type:	HILIC

MS:

MS ID:	MS005076
Analysis ID:	AN005346
Instrument Name:	Thermo Q Exactive Plus Orbitrap
Instrument Type:	Orbitrap
MS Type:	ESI
MS Comments:	The capillary of the electrospray ionization source was set to 275°C, with sheath gas at 45 arbitrary units, auxiliary gas at 5 arbitrary units, and the spray voltage at 4.0 kV. In positive/negative polarity switching mode, a mass/charge ratio (m/z) scan range from 70 to 850 was chosen and MS1 data were collected at a resolution of 70,000. The automatic gain control target was set at 1 × 106, and the maximum injection time was 200 ms. The top five precursor ions were subsequently fragmented, in a data-dependent manner, using the higher-energy collisional dissociation cell set to 30% normalized collision energy in MS2 at a resolution power of 17,500.
Ion Mode:	UNSPECIFIED