Summary of Study ST000165

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 PR000143. The data can be accessed directly via it's Project DOI: 10.21228/M8GP4N This work is supported by NIH grant, U2C- DK119886.

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

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Download additional data:  the amino acids were measured under negative ion chemical ionisation conditions using isobutane as reactant gas

Study ID	ST000165
Study Title	Sparing of muscle mass and function by passive loading in an experimental intensive care unit model
Study Type	time course + intervention
Study Summary	A unique experimental rat ICU model has been used allowing long-term (weeks) time-resolved analyses of the effects of standardized unilateral passive mechanical loading on skeletal muscle size and function and underlying mechanisms. Results show that passive mechanical loading alleviated the muscle wasting and the loss of force-generation associated with the ICU intervention, resulting in a doubling of the functional capacity of the loaded versus the unloaded muscles after a 2-week ICU intervention.
Institute	Uppsala University
Department	Department of Neuroscience
Last Name	Larsson
First Name	Lars
Email	Lars.larsson@neuro.uu.se
Submit Date	2015-05-14
Num Groups	2
Total Subjects	13
Raw Data Available	No
Analysis Type Detail	IR-MS
Release Date	2015-05-10
Release Version	1

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Project:

Project ID:	PR000143
Project DOI:	doi: 10.21228/M8GP4N
Project Title:	Sparing of muscle mass and function by passive loading in an experimental intensive care unit model
Project Summary:	The response to mechanical stimuli, i.e. tensegrity, plays an important role in regulating cell physiological and pathophysiological function, and the mechanical silencing observed in intensive care unit (ICU) patients leads to a severe and specific muscle wasting condition. This study aims to unravel the underlying mechanisms and the effects of passive mechanical loading on skeletal muscle mass and function at the gene, protein and cellular levels. A unique experimental rat ICU model has been used allowing long-term (weeks) time-resolved analyses of the effects of standardized unilateral passive mechanical loading on skeletal muscle size and function and underlying mechanisms. Results show that passive mechanical loading alleviated the muscle wasting and the loss of force-generation associated with the ICU intervention, resulting in a doubling of the functional capacity of the loaded versus the unloaded muscles after a 2-week ICU intervention. We demonstrate that the improved maintenance of muscle mass and function is probably a consequence of a reduced oxidative stress revealed by lower levels of carbonylated proteins, and a reduced loss of the molecular motor protein myosin. A complex temporal gene expression pattern, delineated by microarray analysis, was observed with loading-induced changes in transcript levels of sarcomeric proteins, muscle developmental processes, stress response, extracellular matrix/cell adhesion proteins and metabolism. Thus, the results from this study show that passive mechanical loading alleviates the severe negative consequences on muscle size and function associated with the mechanical silencing in ICU patients, strongly supporting early and intense physical therapy in immobilized ICU patients.
Institute:	Uppsala University
Department:	Department of Neuroscience
Last Name:	Larsson
First Name:	Lars
Email:	Lars.larsson@neuro.uu.se

Subject:

Subject ID:	SU000184
Subject Type:	Animal
Subject Species:	Rattus norvegicus
Taxonomy ID:	10116
Genotype Strain:	SpragueDawley
Gender:	female
Species Group:	Mammal

Factors:

Subject type: Animal; Subject species: Rattus norvegicus (Factor headings shown in green)

mb_sample_id	local_sample_id	Mechanical loading hours/day	Group
SA008938	44	12	Passive Mechanical Loading
SA008939	46	12	Passive Mechanical Loading
SA008940	42	12	Passive Mechanical Loading
SA008941	40	12	Passive Mechanical Loading
SA008942	36	12	Passive Mechanical Loading
SA008943	38	12	Passive Mechanical Loading
SA008944	48	12	Passive Mechanical Loading
SA008945	50	12	Passive Mechanical Loading
SA008946	70	12	Passive Mechanical Loading
SA008947	72	12	Passive Mechanical Loading
SA008948	68	12	Passive Mechanical Loading
SA008949	66	12	Passive Mechanical Loading
SA008950	54	12	Passive Mechanical Loading
SA008951	56	12	Passive Mechanical Loading
SA008952	34	12	Passive Mechanical Loading
SA008953	52	12	Passive Mechanical Loading
SA008954	39	None	Passive Mechanical Loading
SA008955	49	None	Passive Mechanical Loading
SA008956	41	None	Passive Mechanical Loading
SA008957	51	None	Passive Mechanical Loading
SA008958	55	None	Passive Mechanical Loading
SA008959	53	None	Passive Mechanical Loading
SA008960	37	None	Passive Mechanical Loading
SA008961	35	None	Passive Mechanical Loading
SA008962	43	None	Passive Mechanical Loading
SA008963	69	None	Passive Mechanical Loading
SA008964	67	None	Passive Mechanical Loading
SA008965	65	None	Passive Mechanical Loading
SA008966	45	None	Passive Mechanical Loading
SA008967	47	None	Passive Mechanical Loading
SA008968	71	None	Passive Mechanical Loading
SA008969	33	None	Passive Mechanical Loading
SA008970	82	None	Sham
SA008971	81	None	Sham
SA008972	79	None	Sham
SA008973	74	None	Sham
SA008974	73	None	Sham
SA008975	2	None	Sham
SA008976	3	None	Sham
SA008977	75	None	Sham
SA008978	76	None	Sham
SA008979	83	None	Sham
SA008980	78	None	Sham
SA008981	77	None	Sham
SA008982	80	None	Sham
SA008983	85	None	Sham
SA008984	99	None	Sham
SA008985	98	None	Sham
SA008986	97	None	Sham
SA008987	96	None	Sham
SA008988	100	None	Sham
SA008989	101	None	Sham
SA008990	104	None	Sham
SA008991	103	None	Sham
SA008992	102	None	Sham
SA008993	95	None	Sham
SA008994	94	None	Sham
SA008995	88	None	Sham
SA008996	87	None	Sham
SA008997	86	None	Sham
SA008998	4	None	Sham
SA008999	89	None	Sham
SA009000	90	None	Sham
SA009001	93	None	Sham
SA009002	92	None	Sham
SA009003	91	None	Sham
SA009004	84	None	Sham
SA009005	60	None	Sham
SA009006	29	None	Sham
SA009007	28	None	Sham
SA009008	27	None	Sham
SA009009	30	None	Sham
SA009010	31	None	Sham
SA009011	15	None	Sham
SA009012	16	None	Sham
SA009013	32	None	Sham
SA009014	26	None	Sham
SA009015	25	None	Sham
SA009016	20	None	Sham
SA009017	19	None	Sham
SA009018	18	None	Sham
SA009019	21	None	Sham
SA009020	22	None	Sham
SA009021	24	None	Sham
SA009022	23	None	Sham
SA009023	14	None	Sham
SA009024	13	None	Sham
SA009025	17	None	Sham
SA009026	59	None	Sham
SA009027	58	None	Sham
SA009028	61	None	Sham
SA009029	62	None	Sham
SA009030	64	None	Sham
SA009031	63	None	Sham
SA009032	57	None	Sham
SA009033	6	None	Sham
SA009034	10	None	Sham
SA009035	11	None	Sham
SA009036	12	None	Sham
SA009037	9	None	Sham

Showing page 1 of 2 Results: 1 2 Next Showing results 1 to 100 of 104

Collection:

Collection ID:	CO000170
Collection Summary:	The tibialis anterior (TA), extensor digitorum longus (EDL), plantaris, gastrocnemius and soleus muscles were dissected from the loaded left leg and the unloaded right leg immediately after death. One half of the soleus and EDL muscles together with TA and gastrocnemius were quickly frozen in liquid propane cooled by liquid nitrogen, and stored at ?160°C for further analyses. In the other halves of the soleus and EDL muscles, bundles of approximately 50 fibres were dissected from the muscles in relaxing solution at 4°C and tied to glass capillaries, stretched to about 110% of their resting slack length. The bundles were chemically skinned for 24 h in relaxing solution containing 50% (v/v) glycerol for 24 h at 4°C and were subsequently stored at ?20°C (Larsson & Moss, 1993). All the bundles were cryo-protected within 1 week after skinning by transferring the bundles every 30 min to relax solution containing increasing concentrations of sucrose, i.e. 0, 0.5, 1.0, 1.5 and 2.0 m, and subsequently frozen in liquid propane chilled with liquid nitrogen (Frontera & Larsson, 1997). The frozen bundles were stored at ?160°C pending use. One day before the experiments, a bundle was transferred to a 2.0 m sucrose solution for 30 min, subsequently incubated in solutions of decreasing sucrose concentration (1.50.5 m) and finally kept in a skinning solution at ?20°C.
Sample Type:	Muscle

Treatment:

Treatment ID:	TR000190
Treatment Summary:	Mechanical stimulation\|Sham operation
Treatment Protocol Comments:	Sham operated controls and 46 anaesthetized and mechanically ventilated female SpragueDawley rats treated with ?-cobratoxin for durations varying from 6 h to 14 days were included in this study. The experimental model has previously been described in detail (Dworkin & Dworkin, 1990, 2004). For mechanical stimulation animals, left leg was mechanically stimulated and right leg was not. \|Sham operated controls and 46 anaesthetized and mechanically ventilated female SpragueDawley rats treated with ?-cobratoxin for durations varying from 6 h to 14 days were included in this study. The experimental model has previously been described in detail (Dworkin & Dworkin, 1990, 2004). For sham operated controls, no stimulation was performed on either legs

Sample Preparation:

Sampleprep ID:	SP000184
Sampleprep Summary:	An i.v. bolus dose of [ring-13C6]phenylalanine (15 ?g g?1 body weight) was given 15 min prior to the animals being killed. Immediately after death, the gastrocnemius muscle was removed from the left and right hindlimb and split into a medial and lateral deep red and superficial white portion and frozen in liquid propane chilled by liquid nitrogen. Tissue fluid and mixed gastrocnemius muscle proteins were isolated according to the method of Ljungqvist et al. (1997). The mixed muscle protein precipitate from the isolation was hydrolysed by heating with 6 m HCl overnight at 110°C. Both tissue fluid and hydrolysed mixed gastrocnemius muscle amino acids were purified using a BioRad AG-50 × 8 ion exchange resin prior to mass spectrometry analysis. Tissue fluid The level of enrichment of [ring-13C6]phenylalanine in tissue fluid was analysed using ThermoFisher Quantum gas chromatography tandem mass spectrometry (GC/MS/MS) (San Jose, CA, USA). The heptafluorobutyryl isobutyl ester derivative was prepared as described by Ford et al. (1985) and the amino acids were measured under negative ion chemical ionisation conditions using isobutane as reactant gas. The [M-HF]? fragments reflecting the m0 and m+6 species were monitored (m/z transitions 397?377 and 403?383, respectively) and the enrichment of the label was measured against a calibration curve prepared from known amounts of labelled and unlabelled phenylalanine (range 030%).

Sampleprep ID:

SP000184

Sampleprep Summary:

An i.v. bolus dose of [ring-13C6]phenylalanine (15 ?g g?1 body weight) was given 15 min prior to the animals being killed. Immediately after death, the gastrocnemius muscle was removed from the left and right hindlimb and split into a medial and lateral deep red and superficial white portion and frozen in liquid propane chilled by liquid nitrogen. Tissue fluid and mixed gastrocnemius muscle proteins were isolated according to the method of Ljungqvist et al. (1997). The mixed muscle protein precipitate from the isolation was hydrolysed by heating with 6 m HCl overnight at 110°C. Both tissue fluid and hydrolysed mixed gastrocnemius muscle amino acids were purified using a BioRad AG-50 × 8 ion exchange resin prior to mass spectrometry analysis.
Tissue fluid
The level of enrichment of [ring-13C6]phenylalanine in tissue fluid was analysed using ThermoFisher Quantum gas chromatography tandem mass spectrometry (GC/MS/MS) (San Jose, CA, USA). The heptafluorobutyryl isobutyl ester derivative was prepared as described by Ford et al. (1985) and the amino acids were measured under negative ion chemical ionisation conditions using isobutane as reactant gas. The [M-HF]? fragments reflecting the m0 and m+6 species were monitored (m/z transitions 397?377 and 403?383, respectively) and the enrichment of the label was measured against a calibration curve prepared from known amounts of labelled and unlabelled phenylalanine (range 030%).

Combined analysis:

Analysis ID	AN000258
Analysis type	MS
Chromatography type	GC
Chromatography system
Column
MS Type	IR MS
MS instrument type	IR MS
MS instrument name	Thermo DeltaPlus Isotope Ratio MS
Ion Mode	NEGATIVE
Units

Chromatography:

Chromatography ID:	CH000182
Chromatography Summary:	The level of enrichment of [ring-13C6]phenylalanine derived from hydrolysed mixed muscle proteins were analysed using a ThermoFisher DeltaPlus Isotope Ratio mass spectrometer (IR/MS) (Bremen, Germany) fitted with an on-line gas chromatograph with oxidation and reduction furnaces as previously described (Balagopal et al. 1996). The amino acids were derivatized to their trimethyl acetyl, methyl esters according to the method of Metges et al. (1996). Any amino acid eluting from the gas chromatograph is converted to CO2 and N2 prior to entry into the IR/MS. The amino acids were derivatized to their trimethyl acetyl, methyl esters according to the method of Metges et al. (1996). Enrichment of the tracer was measured by monitoring the ratio of 13C to 12CO2 in the IR/MS and again referenced to a calibration curve (00.1%).
Chromatography Type:	GC

MS:

MS ID:	MS000208
Analysis ID:	AN000258
Instrument Name:	Thermo DeltaPlus Isotope Ratio MS
Instrument Type:	IR MS
MS Type:	IR MS
MS Comments:	the amino acids were measured under negative ion chemical ionisation conditions using isobutane as reactant gas
Ion Mode:	NEGATIVE