Paralogs of Atlantic salmon myoblast determination factor genes are distinctly regulated in proliferating and differentiating myogenic cells

The mRNA expression of myogenic regulatory factors, including myoD1 (myoblast determination factor) gene paralogs, and their regulation by amino acids and insulin-like growth factors were investigated in primary cell cultures isolated from fast myotomal muscle of Atlantic salmon (Salmo salar). The c...

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Published in:American Journal of Physiology-Regulatory, Integrative and Comparative Physiology
Main Authors: Bower, Neil I., Johnston, Ian A.
Format: Article in Journal/Newspaper
Language:English
Published: American Physiological Society 2010
Subjects:
Amino acid stimulation
Cell cycle
Genome duplication
Myoblast
myoD
Myogenesis
Subfunctionalization
1314 Physiology
2737 Physiology (medical)
Atlantic salmon
Salmo salar
Online Access:https://espace.library.uq.edu.au/view/UQ:47c5ec0
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spelling ftunivqespace:oai:espace.library.uq.edu.au:UQ:47c5ec0 2023-05-15T15:31:28+02:00 Paralogs of Atlantic salmon myoblast determination factor genes are distinctly regulated in proliferating and differentiating myogenic cells Bower, Neil I. Johnston, Ian A. 2010-06-01 https://espace.library.uq.edu.au/view/UQ:47c5ec0 eng eng American Physiological Society doi:10.1152/ajpregu.00114.2010 issn:0363-6119 issn:1522-1490 orcid:0000-0002-6764-6063 Amino acid stimulation Cell cycle Genome duplication Myoblast myoD Myogenesis Subfunctionalization 1314 Physiology 2737 Physiology (medical) Journal Article 2010 ftunivqespace https://doi.org/10.1152/ajpregu.00114.2010 2020-09-22T02:02:57Z The mRNA expression of myogenic regulatory factors, including myoD1 (myoblast determination factor) gene paralogs, and their regulation by amino acids and insulin-like growth factors were investigated in primary cell cultures isolated from fast myotomal muscle of Atlantic salmon (Salmo salar). The cell cycle and S phase were determined as 28.1 and 13.3 h, respectively, at 18°C. Expression of myoD1b and myoD1c peaked at 8 days of culture in the initial proliferation phase and then declined more than sixfold as cells differentiated and was correlated with PCNA (proliferating cell nuclear antigen) expression (R = 0.88, P < 0.0001; R = 0.70, P < 0.0001). In contrast, myoD1a transcripts increased from 2 to 8 days and remained at elevated levels as myotubes were formed. mRNA levels of myoD1c were, on average, 3.1- and 5.7-fold higher than myoD1a and myoD1b, respectively. Depriving cells of amino acids and serum led to a rapid increase in pax7 and a decrease in myoD1c and PCNA expression, indicating a transition to a quiescent state. In contrast, amino acid replacement in starved cells produced significant increases in myoD1c (at 6 h), PCNA (at 12 h), and myoD1b (at 24 h) and decreases in pax7 expression as cells entered the cell cycle. Our results are consistent with temporally distinct patterns of myoD1c and myoD1b expression at the G and S/G phases of the cell cycle. Treatment of starved cells with insulin-like growth factor I or II did not alter expression of the myoD paralogs. It was concluded that, in vitro, amino acids alone are sufficient to stimulate expression of genes regulating myogenesis in myoblasts involving autocrine/paracrine pathways. The differential responses of myoD paralogs during myotube maturation and amino acid treatments suggest that myoD1b and myoD1c are primarily expressed in proliferating cells and myoD1a in differentiating cells, providing evidence for their subfunctionalization following whole genome and local duplications in the Atlantic salmon lineage. Article in Journal/Newspaper Atlantic salmon Salmo salar The University of Queensland: UQ eSpace American Journal of Physiology-Regulatory, Integrative and Comparative Physiology 298 6 R1615 R1626
institution Open Polar
collection The University of Queensland: UQ eSpace
op_collection_id ftunivqespace
language English
topic Amino acid stimulation
Cell cycle
Genome duplication
Myoblast
myoD
Myogenesis
Subfunctionalization
1314 Physiology
2737 Physiology (medical)
spellingShingle Amino acid stimulation
Cell cycle
Genome duplication
Myoblast
myoD
Myogenesis
Subfunctionalization
1314 Physiology
2737 Physiology (medical)
Bower, Neil I.
Johnston, Ian A.
Paralogs of Atlantic salmon myoblast determination factor genes are distinctly regulated in proliferating and differentiating myogenic cells
topic_facet Amino acid stimulation
Cell cycle
Genome duplication
Myoblast
myoD
Myogenesis
Subfunctionalization
1314 Physiology
2737 Physiology (medical)
description The mRNA expression of myogenic regulatory factors, including myoD1 (myoblast determination factor) gene paralogs, and their regulation by amino acids and insulin-like growth factors were investigated in primary cell cultures isolated from fast myotomal muscle of Atlantic salmon (Salmo salar). The cell cycle and S phase were determined as 28.1 and 13.3 h, respectively, at 18°C. Expression of myoD1b and myoD1c peaked at 8 days of culture in the initial proliferation phase and then declined more than sixfold as cells differentiated and was correlated with PCNA (proliferating cell nuclear antigen) expression (R = 0.88, P < 0.0001; R = 0.70, P < 0.0001). In contrast, myoD1a transcripts increased from 2 to 8 days and remained at elevated levels as myotubes were formed. mRNA levels of myoD1c were, on average, 3.1- and 5.7-fold higher than myoD1a and myoD1b, respectively. Depriving cells of amino acids and serum led to a rapid increase in pax7 and a decrease in myoD1c and PCNA expression, indicating a transition to a quiescent state. In contrast, amino acid replacement in starved cells produced significant increases in myoD1c (at 6 h), PCNA (at 12 h), and myoD1b (at 24 h) and decreases in pax7 expression as cells entered the cell cycle. Our results are consistent with temporally distinct patterns of myoD1c and myoD1b expression at the G and S/G phases of the cell cycle. Treatment of starved cells with insulin-like growth factor I or II did not alter expression of the myoD paralogs. It was concluded that, in vitro, amino acids alone are sufficient to stimulate expression of genes regulating myogenesis in myoblasts involving autocrine/paracrine pathways. The differential responses of myoD paralogs during myotube maturation and amino acid treatments suggest that myoD1b and myoD1c are primarily expressed in proliferating cells and myoD1a in differentiating cells, providing evidence for their subfunctionalization following whole genome and local duplications in the Atlantic salmon lineage.
format Article in Journal/Newspaper
author Bower, Neil I.
Johnston, Ian A.
author_facet Bower, Neil I.
Johnston, Ian A.
author_sort Bower, Neil I.
title Paralogs of Atlantic salmon myoblast determination factor genes are distinctly regulated in proliferating and differentiating myogenic cells
title_short Paralogs of Atlantic salmon myoblast determination factor genes are distinctly regulated in proliferating and differentiating myogenic cells
title_full Paralogs of Atlantic salmon myoblast determination factor genes are distinctly regulated in proliferating and differentiating myogenic cells
title_fullStr Paralogs of Atlantic salmon myoblast determination factor genes are distinctly regulated in proliferating and differentiating myogenic cells
title_full_unstemmed Paralogs of Atlantic salmon myoblast determination factor genes are distinctly regulated in proliferating and differentiating myogenic cells
title_sort paralogs of atlantic salmon myoblast determination factor genes are distinctly regulated in proliferating and differentiating myogenic cells
publisher American Physiological Society
publishDate 2010
url https://espace.library.uq.edu.au/view/UQ:47c5ec0
genre Atlantic salmon
Salmo salar
genre_facet Atlantic salmon
Salmo salar
op_relation doi:10.1152/ajpregu.00114.2010
issn:0363-6119
issn:1522-1490
orcid:0000-0002-6764-6063
op_doi https://doi.org/10.1152/ajpregu.00114.2010
container_title American Journal of Physiology-Regulatory, Integrative and Comparative Physiology
container_volume 298
container_issue 6
container_start_page R1615
op_container_end_page R1626
_version_ 1766361986386362368

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