Different Resistance Exercise Loading Paradigms Similarly Affect Skeletal Muscle Gene Expression Patterns of Myostatin-Related Targets and mTORC1 Signaling Markers.

dc.contributor.author

McIntosh, Mason C

dc.contributor.author

Sexton, Casey L

dc.contributor.author

Godwin, Joshua S

dc.contributor.author

Ruple, Bradley A

dc.contributor.author

Michel, J Max

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Plotkin, Daniel L

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Ziegenfuss, Tim N

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Lopez, Hector L

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Smith, Ryan

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Dwaraka, Varun B

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Sharples, Adam P

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Dalbo, Vincent J

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Mobley, C Brooks

dc.contributor.author

Vann, Christopher G

dc.contributor.author

Roberts, Michael D

dc.date.accessioned

2024-01-11T17:18:32Z

dc.date.available

2024-01-11T17:18:32Z

dc.date.issued

2023-03

dc.description.abstract

Although transcriptome profiling has been used in several resistance training studies, the associated analytical approaches seldom provide in-depth information on individual genes linked to skeletal muscle hypertrophy. Therefore, a secondary analysis was performed herein on a muscle transcriptomic dataset we previously published involving trained college-aged men (n = 11) performing two resistance exercise bouts in a randomized and crossover fashion. The lower-load bout (30 Fail) consisted of 8 sets of lower body exercises to volitional fatigue using 30% one-repetition maximum (1 RM) loads, whereas the higher-load bout (80 Fail) consisted of the same exercises using 80% 1 RM loads. Vastus lateralis muscle biopsies were collected prior to (PRE), 3 h, and 6 h after each exercise bout, and 58 genes associated with skeletal muscle hypertrophy were manually interrogated from our prior microarray data. Select targets were further interrogated for associated protein expression and phosphorylation induced-signaling events. Although none of the 58 gene targets demonstrated significant bout x time interactions, ~57% (32 genes) showed a significant main effect of time from PRE to 3 h (15↑ and 17↓, p < 0.01), and ~26% (17 genes) showed a significant main effect of time from PRE to 6 h (8↑ and 9↓, p < 0.01). Notably, genes associated with the myostatin (9 genes) and mammalian target of rapamycin complex 1 (mTORC1) (9 genes) signaling pathways were most represented. Compared to mTORC1 signaling mRNAs, more MSTN signaling-related mRNAs (7 of 9) were altered post-exercise, regardless of the bout, and RHEB was the only mTORC1-associated mRNA that was upregulated following exercise. Phosphorylated (phospho-) p70S6K (Thr389) (p = 0.001; PRE to 3 h) and follistatin protein levels (p = 0.021; PRE to 6 h) increased post-exercise, regardless of the bout, whereas phospho-AKT (Thr389), phospho-mTOR (Ser2448), and myostatin protein levels remained unaltered. These data continue to suggest that performing resistance exercise to volitional fatigue, regardless of load selection, elicits similar transient mRNA and signaling responses in skeletal muscle. Moreover, these data provide further evidence that the transcriptional regulation of myostatin signaling is an involved mechanism in response to resistance exercise.

dc.identifier

cells12060898

dc.identifier.issn

2073-4409

dc.identifier.issn

2073-4409

dc.identifier.uri

https://hdl.handle.net/10161/29753

dc.language

eng

dc.publisher

MDPI AG

dc.relation.ispartof

Cells

dc.relation.isversionof

10.3390/cells12060898

dc.rights.uri

https://creativecommons.org/licenses/by-nc/4.0

dc.subject

Muscle, Skeletal

dc.subject

Humans

dc.subject

Hypertrophy

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RNA, Messenger

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Gene Expression

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Male

dc.subject

Resistance Training

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Myostatin

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Young Adult

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Mechanistic Target of Rapamycin Complex 1

dc.title

Different Resistance Exercise Loading Paradigms Similarly Affect Skeletal Muscle Gene Expression Patterns of Myostatin-Related Targets and mTORC1 Signaling Markers.

dc.type

Journal article

pubs.begin-page

898

pubs.issue

6

pubs.organisational-group

Duke

pubs.organisational-group

School of Medicine

pubs.organisational-group

Staff

pubs.organisational-group

Institutes and Centers

pubs.organisational-group

Center for the Study of Aging and Human Development

pubs.publication-status

Published

pubs.volume

12

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