Summary of Study ST001810

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 PR001144. The data can be accessed directly via it's Project DOI: 10.21228/M8TQ3Q 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	ST001810
Study Title	Metabolomics-driven identification of biochemical mechanisms underlying the neuroprotective effects of pleiotrophin in a mouse model of Parkinson’s disease
Study Summary	Pleiotrophin (PTN) is a cytokine involved in nerve tissue repair processes, neuroinflammation and neuronal survival. PTN expression levels are upregulated in the nigrostriatal pathway of Parkinson’s Disease (PD) patients. We aimed to characterize the dopaminergic injury and glial activation in the nigrostriatal pathway of mice with transgenic Ptn overexpression in the brain (Ptn-Tg) after intrastriatal injection of the Parkinsonian toxin 6-hydroxydopamine (6-OHDA). The injection of 6-OHDA induced a significant decrease of the number of tyrosine hydroxylase (TH)-positive neurons in the substantia nigra and of the striatal TH contents in Wild type (Wt) mice. In contrast, these effects of 6-OHDA were blocked in Ptn-Tg mice. 6-OHDA injection did not cause robust changes in microglia but induced an exacerbated astrocytic response in Wt mice compared with Ptn-Tg mice. In metabolomics studies, we detected interesting metabolites that significantly discriminate the more injured 6-OHDA-injected Wt striatum and the more protected 6-OHDA-injected Ptn-Tg striatum. Particularly, we detected groups of metabolites, mostly corresponding to phospholipids, whose trends were opposite in both groups. In summary, the data confirm the neuroprotective effect of brain PTN overexpression in this mouse model of PD. New lipid-related PD drug candidates emerge from this study and the data presented here support the increasingly recognized “lipid cascade” in PD.
Institute	CEMBIO
Last Name	Sáiz
First Name	Jorge
Address	JULIÁN ROMEA 23, Madrid, Madrid, 28003, Spain
Email	jorge.saizgalindo@ceu.es
Phone	none
Submit Date	2021-06-01
Raw Data Available	Yes
Raw Data File Type(s)	d
Analysis Type Detail	LC-MS
Release Date	2021-06-16
Release Version	1

Select appropriate tab below to view additional metadata details:

Project:

Project ID:	PR001144
Project DOI:	doi: 10.21228/M8TQ3Q
Project Title:	Metabolomics-driven identification of biochemical mechanisms underlying the neuroprotective effects of pleiotrophin in a mouse model of Parkinson’s disease
Project Summary:	Pleiotrophin (PTN) is a cytokine involved in nerve tissue repair processes, neuroinflammation and neuronal survival. PTN expression levels are upregulated in the nigrostriatal pathway of Parkinson’s Disease (PD) patients. We aimed to characterize the dopaminergic injury and glial activation in the nigrostriatal pathway of mice with transgenic Ptn overexpression in the brain (Ptn-Tg) after intrastriatal injection of the Parkinsonian toxin 6-hydroxydopamine (6-OHDA). The injection of 6-OHDA induced a significant decrease of the number of tyrosine hydroxylase (TH)-positive neurons in the substantia nigra and of the striatal TH contents in Wild type (Wt) mice. In contrast, these effects of 6-OHDA were blocked in Ptn-Tg mice. 6-OHDA injection did not cause robust changes in microglia but induced an exacerbated astrocytic response in Wt mice compared with Ptn-Tg mice. In metabolomics studies, we detected interesting metabolites that significantly discriminate the more injured 6-OHDA-injected Wt striatum and the more protected 6-OHDA-injected Ptn-Tg striatum. Particularly, we detected groups of metabolites, mostly corresponding to phospholipids, whose trends were opposite in both groups. In summary, the data confirm the neuroprotective effect of brain PTN overexpression in this mouse model of PD. New lipid-related PD drug candidates emerge from this study and the data presented here support the increasingly recognized “lipid cascade” in PD.
Institute:	Universidad CEU San Pablo
Last Name:	Sáiz
First Name:	Jorge
Address:	JULIÁN ROMEA 23, Madrid, Madrid, 28003, Spain
Email:	jorge.saizgalindo@ceu.es
Phone:	913 72 47 11

Subject:

Subject ID:	SU001887
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	Subject type	Treatment
SA168132	QC5-POS	QC	QC
SA168133	QC6-POS	QC	QC
SA168134	QC4-POS	QC	QC
SA168135	QC2-POS	QC	QC
SA168136	QC1-POS	QC	QC
SA168137	QC1-NEG	QC	QC
SA168138	QC3-POS	QC	QC
SA168139	QC7-POS	QC	QC
SA168140	QC6-NEG	QC	QC
SA168141	QC7-NEG	QC	QC
SA168142	QC4-NEG	QC	QC
SA168143	QC5-NEG	QC	QC
SA168144	QC3-NEG	QC	QC
SA168145	QC2-NEG	QC	QC
SA168146	T3-HD-NEG.d	Transg	OH-Dopamine
SA168147	T2-HD-NEG.d	Transg	OH-Dopamine
SA168148	T1-HD-NEG.d	Transg	OH-Dopamine
SA168149	T5-HD-NEG.d	Transg	OH-Dopamine
SA168150	T4-HD-NEG.d	Transg	OH-Dopamine
SA168151	T2-HD-POS.d	Transg	OH-Dopamine
SA168152	T3-HD-POS.d	Transg	OH-Dopamine
SA168153	T4-HD-POS.d	Transg	OH-Dopamine
SA168154	T1-HD-POS.d	Transg	OH-Dopamine
SA168155	T5-HD-POS.d	Transg	OH-Dopamine
SA168156	T1-VEH-NEG.d	Transg	Vehicle
SA168157	T7-VEH-NEG.d	Transg	Vehicle
SA168158	T6-VEH-NEG.d	Transg	Vehicle
SA168159	T5-VEH-NEG.d	Transg	Vehicle
SA168160	T6-VEH-POS.d	Transg	Vehicle
SA168161	T7-VEH-POS.d	Transg	Vehicle
SA168162	T4-VEH-NEG.d	Transg	Vehicle
SA168163	T5-VEH-POS.d	Transg	Vehicle
SA168164	T1-VEH-POS.d	Transg	Vehicle
SA168165	T2-VEH-NEG.d	Transg	Vehicle
SA168166	T2-VEH-POS.d	Transg	Vehicle
SA168167	T4-VEH-POS.d	Transg	Vehicle
SA168168	WT8-HD-NEG.d	WT	OH-Dopamine
SA168169	WT7-HD-NEG.d	WT	OH-Dopamine
SA168170	WT9-HD-NEG.d	WT	OH-Dopamine
SA168171	WT11-HD-NEG.d	WT	OH-Dopamine
SA168172	WT6-HD-NEG.d	WT	OH-Dopamine
SA168173	WT12-HD-NEG.d	WT	OH-Dopamine
SA168174	WT10-HD-NEG.d	WT	OH-Dopamine
SA168175	WT1-HD-NEG.d	WT	OH-Dopamine
SA168176	WT9-HD-POS.d	WT	OH-Dopamine
SA168177	WT8-HD-POS.d	WT	OH-Dopamine
SA168178	WT7-HD-POS.d	WT	OH-Dopamine
SA168179	WT10-HD-POS.d	WT	OH-Dopamine
SA168180	WT11-HD-POS.d	WT	OH-Dopamine
SA168181	WT5-HD-NEG.d	WT	OH-Dopamine
SA168182	WT12-HD-POS.d	WT	OH-Dopamine
SA168183	WT5-HD-POS.d	WT	OH-Dopamine
SA168184	WT6-HD-POS.d	WT	OH-Dopamine
SA168185	WT3-HD-NEG.d	WT	OH-Dopamine
SA168186	WT4-HD-NEG.d	WT	OH-Dopamine
SA168187	WT2-HD-NEG.d	WT	OH-Dopamine
SA168188	WT1-HD-POS.d	WT	OH-Dopamine
SA168189	WT4-HD-POS.d	WT	OH-Dopamine
SA168190	WT3-HD-POS.d	WT	OH-Dopamine
SA168191	WT2-HD-POS.d	WT	OH-Dopamine
SA168192	WT2-VEH-POS.d	WT	Vehicle
SA168193	WT1-VEH-POS.d	WT	Vehicle
SA168194	WT3-VEH-POS.d	WT	Vehicle
SA168195	WT7-VEH-NEG.d	WT	Vehicle
SA168196	WT6-VEH-POS.d	WT	Vehicle
SA168197	WT4-VEH-POS.d	WT	Vehicle
SA168198	WT7-VEH-POS.d	WT	Vehicle
SA168199	WT8-VEH-POS.d	WT	Vehicle
SA168200	WT10-VEH-POS.d	WT	Vehicle
SA168201	WT9-VEH-POS.d	WT	Vehicle
SA168202	WT1-VEH-NEG.d	WT	Vehicle
SA168203	WT2-VEH-NEG.d	WT	Vehicle
SA168204	WT8-VEH-NEG.d	WT	Vehicle
SA168205	WT9-VEH-NEG.d	WT	Vehicle
SA168206	WT6-VEH-NEG.d	WT	Vehicle
SA168207	WT4-VEH-NEG.d	WT	Vehicle
SA168208	WT3-VEH-NEG.d	WT	Vehicle
SA168209	WT10-VEH-NEG.d	WT	Vehicle

Showing results 1 to 78 of 78

Showing results 1 to 78 of 78

Collection:

Collection ID:	CO001880
Collection Summary:	Samples were collected and frozen at -80ºC
Sample Type:	Brain

Treatment:

Treatment ID:	TR001900
Treatment Summary:	Striatum resections were added to 300 µL MeOH:water (50:50) in 2 mL Eppendorf tubes and were first homogenized with glass beads in a TissueLyser LT (QIAGEN) for 2 min. The tubes were immersed in liquid N2 and homogenized again in the TissueLyser LT for another 2 min. A volume 100 µL of the homogenate was transferred into Eppendorf tubes of 1.5 mL and added with 320 µL of methanol and 80 µL of MTBE and the mixture was vortexed for 1 h. Afterwards, the vials were centrifuged at 4000 g for 20 min at 20 ºC and 300 µL of the supernatants were transferred into new tubes, which were evaporated to dryness in a vacuum concentrator. Finally, the residues were reconstituted in 50 µL of MeOH:water:MTBE (37:5:4), being the samples ready for their analysis. Blank samples were prepared following the sample procedure without the addition of any biological tissue.

Treatment ID:

TR001900

Treatment Summary:

Striatum resections were added to 300 µL MeOH:water (50:50) in 2 mL Eppendorf tubes and were first homogenized with glass beads in a TissueLyser LT (QIAGEN) for 2 min. The tubes were immersed in liquid N2 and homogenized again in the TissueLyser LT for another 2 min. A volume 100 µL of the homogenate was transferred into Eppendorf tubes of 1.5 mL and added with 320 µL of methanol and 80 µL of MTBE and the mixture was vortexed for 1 h. Afterwards, the vials were centrifuged at 4000 g for 20 min at 20 ºC and 300 µL of the supernatants were transferred into new tubes, which were evaporated to dryness in a vacuum concentrator. Finally, the residues were reconstituted in 50 µL of MeOH:water:MTBE (37:5:4), being the samples ready for their analysis. Blank samples were prepared following the sample procedure without the addition of any biological tissue.

Sample Preparation:

Sampleprep ID:	SP001893
Sampleprep Summary:	Striatum resections were added to 300 µL MeOH:water (50:50) in 2 mL Eppendorf tubes and were first homogenized with glass beads in a TissueLyser LT (QIAGEN) for 2 min. The tubes were immersed in liquid N2 and homogenized again in the TissueLyser LT for another 2 min. A volume 100 µL of the homogenate was transferred into Eppendorf tubes of 1.5 mL and added with 320 µL of methanol and 80 µL of MTBE and the mixture was vortexed for 1 h. Afterwards, the vials were centrifuged at 4000 g for 20 min at 20 ºC and 300 µL of the supernatants were transferred into new tubes, which were evaporated to dryness in a vacuum concentrator. Finally, the residues were reconstituted in 50 µL of MeOH:water:MTBE (37:5:4), being the samples ready for their analysis. Blank samples were prepared following the sample procedure without the addition of any biological tissue.

Sampleprep ID:

SP001893

Sampleprep Summary:

Combined analysis:

Analysis ID	AN002933	AN002934
Analysis type	MS	MS
Chromatography type	Reversed phase	Reversed phase
Chromatography system	Agilent 1200	Agilent 1200
Column	RP C8 Agilent Poroshell (150 x 2.1mm,2.7um)	RP C8 Agilent Poroshell (150 x 2.1mm,2.7um)
MS Type	ESI	ESI
MS instrument type	QTOF	QTOF
MS instrument name	Agilent 6520 QTOF	Agilent 6520 QTOF
Ion Mode	POSITIVE	NEGATIVE
Units	aera	area

Chromatography:

Chromatography ID:	CH002174
Instrument Name:	Agilent 1200
Column Name:	RP C8 Agilent Poroshell (150 x 2.1mm,2.7um)
Chromatography Type:	Reversed phase

MS:

MS ID:	MS002724
Analysis ID:	AN002933
Instrument Name:	Agilent 6520 QTOF
Instrument Type:	QTOF
MS Type:	ESI
MS Comments:	All data were controlled and acquired using Mass Hunter Qualitative Analysis B.07.00 (Agilent Technologies). Data obtained from LC-MS were cleaned of background noise and unrelated ions. Peak detection, deconvolution and alignment were performed by the recursive feature extraction (RFE) using Profinder Software B.08.00 (Agilent Technologies). Blank subtraction and filtering by frequency of at least 50% of the QC and 60% of each group and relative standard deviation (RSD) less than 30% in QC were performed, to keep only the relevant features. Missing values were substituted by KNN algorithm.
Ion Mode:	POSITIVE

MS ID:	MS002725
Analysis ID:	AN002934
Instrument Name:	Agilent 6520 QTOF
Instrument Type:	QTOF
MS Type:	ESI
MS Comments:	All data were controlled and acquired using Mass Hunter Qualitative Analysis B.07.00 (Agilent Technologies). Data obtained from LC-MS were cleaned of background noise and unrelated ions. Peak detection, deconvolution and alignment were performed by the recursive feature extraction (RFE) using Profinder Software B.08.00 (Agilent Technologies). Blank subtraction and filtering by frequency of at least 50% of the QC and 60% of each group and relative standard deviation (RSD) less than 30% in QC were performed, to keep only the relevant features. Missing values were substituted by KNN algorithm.
Ion Mode:	NEGATIVE