Summary of Study ST001907

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 PR001201. The data can be accessed directly via it's Project DOI: 10.21228/M8G69Q 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	ST001907
Study Title	Training-induced bioenergetic improvement in human skeletal muscle is associated with non-stoichiometric changes in the mitochondrial proteome without reorganisation of respiratory chain content
Study Type	Multi Omics
Study Summary	Lipidomic analysis of muscle mitochondrial isolates. 10 men with repeated measures.
Institute	Baker Heart and Diabetes Institute
Department	Meteabolomics
Laboratory	Meteabolomics
Last Name	Huynh
First Name	Kevin
Address	75 Commercial Road
Email	kevin.huynh@baker.edu.au
Phone	0385321537
Submit Date	2021-08-15
Num Groups	1
Total Subjects	10
Num Males	10
Raw Data Available	Yes
Raw Data File Type(s)	mzML
Analysis Type Detail	LC-MS
Release Date	2021-10-18
Release Version	1

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Project:

Project ID:	PR001201
Project DOI:	doi: 10.21228/M8G69Q
Project Title:	Training-induced bioenergetic improvement in human skeletal muscle is associated with non-stoichiometric changes in the mitochondrial proteome without reorganisation of respiratory chain content
Project Type:	Multi-omics
Project Summary:	Defects in mitochondria have been implicated in multiple diseases and aging. Interventions to improve mitochondrial function have the potential to improve quality of life. Exercise training is a readily accessible and inexpensive intervention, however how it promotes mitochondrial adaptation in skeletal muscle remains poorly understood. Here, we describe an intricate and previously undemonstrated network of differentially prioritised training-induced adaptations in human skeletal muscle mitochondria. We show that changes in hundreds of transcripts, proteins and lipid species are not stoichiometrically linked to the increase in mitochondrial content. We demonstrate a prioritization of specific pathways at different stages of the intervention, including initial deprioritisation of oxidative phosphorylation (OXPHOS) and prioritisation of TCA cycle and fatty acid β-oxidation linked mitochondrial respiration. This indicates that enhancing electron flow to OXPHOS is more important to increase ATP production than increasing the abundance of the OXPHOS machinery. Our research unearths the elaborate and multi-layered nature of the adaptive response to exercise and provides a valuable resource that can be mined to maximise the therapeutic benefits of exercise.
Institute:	Baker Heart and Diabetes Institute
Department:	Baker Heart and Diabetes Institute
Laboratory:	Metabolomics
Last Name:	Huynh
First Name:	Kevin
Address:	75 Commercial Road
Email:	kevin.huynh@baker.edu.au
Phone:	0385321537

Subject:

Subject ID:	SU001985
Subject Type:	Human
Subject Species:	Homo sapiens
Taxonomy ID:	9606
Gender:	Male

Factors:

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

mb_sample_id	local_sample_id	ID
SA176734	10NK-1	0N
SA176735	10NK-2	0N
SA176736	10NK-8	0N
SA176737	10NK-5	0N
SA176738	12JP-8	2J
SA176739	12JP-2	2J
SA176740	12JP-1	2J
SA176741	12JP-5	2J
SA176742	13AP-1	3A
SA176743	13AP-5	3A
SA176744	13AP-8	3A
SA176745	13AP-2	3A
SA176746	14EP-8	4E
SA176747	14EP-1	4E
SA176748	14EP-2	4E
SA176749	14EP-5	4E
SA176750	1AM-2	AM
SA176751	1AM-5	AM
SA176752	1AM-1	AM
SA176753	1AM-8	AM
SA176754	5CP-2	CP
SA176755	5CP-1	CP
SA176756	5CP-8	CP
SA176757	5CP-5	CP
SA176758	9GG-1	GG
SA176759	9GG-2	GG
SA176760	9GG-5	GG
SA176761	9GG-8	GG
SA176762	7SL-8	SL
SA176763	7SL-1	SL
SA176764	7SL-5	SL
SA176765	7SL-2	SL
SA176766	4SR-2	SR
SA176767	4SR-8	SR
SA176768	4SR-1	SR
SA176769	4SR-5	SR
SA176770	6WP-2	WP
SA176771	6WP-8	WP
SA176772	6WP-1	WP
SA176773	6WP-5	WP

Showing results 1 to 40 of 40

Showing results 1 to 40 of 40

Collection:

Collection ID:	CO001978
Collection Summary:	Muscle biopsies. A biopsy needle with suction under local anaesthesia (1% xylocaine) was 688 used to obtain vastus lateralis muscle biopsies at rest at the following four time points: BL, 689 PN, PH and PR. After being cleaned of excess blood, connective and fat tissue muscle 690 biopsies were divided as follows: ~10 mg was immediately immersed in ~2 mL of ice-cold 691 BIOPS for measurements of mitochondrial respiration, whereas the remainder was promptly 692 frozen in liquid nitrogen and stored at -80°C for follow-up analyses.
Sample Type:	Muscle

Treatment:

Treatment ID:	TR001997
Treatment Summary:	Training intervention. All training sessions were performed on an electronically braked cycle ergometer (Velotron, RacerMate, USA), following an 8-min warm up (see 20k-TT) and consisted of HIIT (2:1 work-to-rest ratio). Training intensity was set relative to ẆLT (rather than ẆPeak) so as to induce similar metabolic and cardiac stresses amongst participants of differing fitness levels75. Exercise intensity was maintained between ẆLT and ẆPeak throughout the entire study so that training volume was the only manipulated variable between the 3 phases. NVT phase. This consisted of 6 HIIT sessions within 2 weeks of 5 to 7 4-min cycling intervals interspersed with a 2-min recovery at 60 W. Exercise intensities were defined as [ẆLT + x(ẆPeak-ẆLT)], with x increasing from 0.5 to 0.7 throughout the phase. HVT phase. Participants performed HIIT twice a day for 20 consecutive days; training sessions consisted of either 7 to 10 4-min intervals interspersed with a 2-min recovery at 60 W at intensities ranging from [ẆLT + 0.5(ẆPeak-ẆLT)] to [ẆLT + 0.8(ẆPeak-ẆLT)], or 15 to 20 2-min intervals at intensities ranging from [ẆLT + 0.5(ẆPeak-ẆLT)] to [ẆLT + 0.95(ẆPeak-ẆLT)], interspersed with a 1-min recovery at 60 W. Single session duration increased from ~45 min to 60 min. RVT phase. The RVT phase consisted of 6 HIIT sessions in 6 days; participants performed 10, 9, 8, 7, 6, and 4, 4-min intervals interspersed with a 2-min recovery at 60 W, at an intensity of [ẆLT + x(ẆPeak- ẆLT)], with x increasing from 0.5 to 0.7 throughout the phase.

Treatment ID:

TR001997

Treatment Summary:

Training intervention. All training sessions were performed on an electronically braked cycle ergometer (Velotron, RacerMate, USA), following an 8-min warm up (see 20k-TT) and consisted of HIIT (2:1 work-to-rest ratio). Training intensity was set relative to ẆLT (rather than ẆPeak) so as to induce similar metabolic and cardiac stresses amongst participants of differing fitness levels75. Exercise intensity was maintained between ẆLT and ẆPeak throughout the entire study so that training volume was the only manipulated variable between the 3 phases. NVT phase. This consisted of 6 HIIT sessions within 2 weeks of 5 to 7 4-min cycling intervals interspersed with a 2-min recovery at 60 W. Exercise intensities were defined as [ẆLT + x(ẆPeak-ẆLT)], with x increasing from 0.5 to 0.7 throughout the phase. HVT phase. Participants performed HIIT twice a day for 20 consecutive days; training sessions consisted of either 7 to 10 4-min intervals interspersed with a 2-min recovery at 60 W at intensities ranging from [ẆLT + 0.5(ẆPeak-ẆLT)] to [ẆLT + 0.8(ẆPeak-ẆLT)], or 15 to 20 2-min intervals at intensities ranging from [ẆLT + 0.5(ẆPeak-ẆLT)] to [ẆLT + 0.95(ẆPeak-ẆLT)], interspersed with a 1-min recovery at 60 W. Single session duration increased from ~45 min to 60 min. RVT phase. The RVT phase consisted of 6 HIIT sessions in 6 days; participants performed 10, 9, 8, 7, 6, and 4, 4-min intervals interspersed with a 2-min recovery at 60 W, at an intensity of [ẆLT + x(ẆPeak- ẆLT)], with x increasing from 0.5 to 0.7 throughout the phase.

Sample Preparation:

Sampleprep ID:	SP001991
Sampleprep Summary:	Mitochondrial isolates were extracted using a modified single-phase chloroform/methanol extraction as described previously (Weir et al. 2013). In brief, 20 volumes of chloroform:methanol (2:1) were added to the sample along with a series of internal standards. Samples were vortexed and centrifuged on a rotary mixer for 10 min. Following sonication on a sonicator bath for 30 min, samples were rested for 20 min prior to centrifugation at 13,000 g for 10 min. Supernatants were transferred into a 96 well plated, dried down and reconstituted in 50 μL H2O saturated butanol and sonicated for 10 min. After the addition of 50 μL of methanol with 10 mM ammonium 945 formate, samples were centrifuged at 4000 rpm on a plate centrifuge and transferred into glass vials with inserts for mass spectrometry analysis.
Processing Storage Conditions:	-80℃
Extraction Method:	Single phase 2:1 chloroform methanol
Extract Storage:	-80℃
Sample Resuspension:	Butanol : Methanol 1:1
Subcellular Location:	Mitochondria

Combined analysis:

Analysis ID	AN003104
Analysis type	MS
Chromatography type	Reversed phase
Chromatography system	Agilent 1290 Infinity II
Column	Agilent Zorbax Eclipse Plus C18 (100 x 2.1mm, 1.8 um)
MS Type	ESI
MS instrument type	Triple quadrupole
MS instrument name	Agilent 6490 QQQ
Ion Mode	POSITIVE
Units	pmol per mg

Chromatography:

Chromatography ID:	CH002291
Chromatography Summary:	The running solvent consisted of solvent A: 50% H2O / 30% acetonitrile / 20% isopropanol (v/v/v) containing 10mM ammonium formate and 5uM medronic acid, and solvent B: 1% H2O / 9% acetonitrile / 90% isopropanol (v/v/v) containing 10mM ammonium formate. We utilized a stepped linear gradient with a 16-minute cycle time per sample and a 1µL sample injection. To increase throughput, we used a dual column set up to equilibrate the second column while the first is running a sample. The sample analytical gradient was as follows: starting with a flow rate of 0.4mL/minute at 15% B and increasing to 50% B over 2.5 minutes, then to 57% over 0.1 minutes, to 70% over 6.4 minutes, to 93% over 0.1 minute, to 96% over 1.9 minutes and finally to 100% over 0.1 minute. The solvent was then held at 100% B for 0.9 minutes (total 12.0 minutes). Equilibration was started as follows: solvent was decreased from 100% B to 15% B over 0.2 minutes and held until a total of 16 minutes. The next sample is injected and the columns are switched.
Instrument Name:	Agilent 1290 Infinity II
Column Name:	Agilent Zorbax Eclipse Plus C18 (100 x 2.1mm, 1.8 um)
Flow Gradient:	starting with a flow rate of 0.4mL/minute at 15% B and increasing to 50% B over 2.5 minutes, then to 57% over 0.1 minutes, to 70% over 6.4 minutes, to 93% over 0.1 minute, to 96% over 1.9 minutes and finally to 100% over 0.1 minute. The solvent was then held at 100% B for 0.9 minutes (total 12.0 minutes). Equilibration was started as follows: solvent was decreased from 100% B to 15% B over 0.2 minutes and held until a total of 16 minutes.
Flow Rate:	0.4mL/min
Solvent A:	50% water/30% acetonitrile/20% isopropanol; 10mM ammonium formate; 5uM medronic acid
Solvent B:	1% water/9% acetonitrile/90% isopropanol; 10mM ammonium formate
Chromatography Type:	Reversed phase

MS:

MS ID:	MS002886
Analysis ID:	AN003104
Instrument Name:	Agilent 6490 QQQ
Instrument Type:	Triple quadrupole
MS Type:	ESI
MS Comments:	Details previously published in https://doi.org/10.1016/j.chembiol.2018.10.008
Ion Mode:	POSITIVE