Variation in protein abundance profiles in the M. semitendinosus of lambs bred from sires selected on the basis of growth and muscling potential
M. B. McDonagh A E , K. L. Ferguson B , A. Bacic B , G. E. Gardner C and R. S. Hegarty DA Victorian Department of Primary Industries, Werribee, Vic. 3030, Australia.
B Australian Centre for Plant Functional Genomics and Plant Cell Biology Research Centre, School of Botany, The University of Melbourne, Vic. 3010, Australia.
C University of New England, Armidale, NSW 2351, Australia.
D NSW Department of Primary Industries, Beef Industry Centre of Excellence, Armidale, NSW 2351, Australia.
E Corresponding author. Email: Matthew.McDonagh@dpi.vic.gov.au
Australian Journal of Agricultural Research 57(6) 671-682 https://doi.org/10.1071/AR04277
Submitted: 16 November 2004 Accepted: 7 December 2005 Published: 20 June 2006
Abstract
Relative abundance of proteins localised in the nuclear-enriched, total cell membrane and cytosolic fractions of the semitendinosus muscle was compared between lambs bred from control (C), high muscling (M), and high growth rate (G) sires. In total, 31 proteins were identified whose abundance was differentially regulated between sire type. Differences in hind-limb muscle development between M lambs and C and G lambs were reflected in levels of proteins that regulate or function in cellular mechanisms of protein and energy metabolism. Despite no apparent difference in hind-limb muscle growth in G lambs compared to C, G lambs exhibited marked differences in proteins involved in regulation and function of energy metabolism. These results detail pathways that can be specifically targeted to enhance muscle accretion and growth in lambs. The development of means to manipulate these cellular mechanisms may yield greater gains in muscle accretion and growth rate than breeding on the basis for genetic capacity alone.
Additional keywords: proteomics, proteome, skeletal muscle, sheep, expression, two-dimensional electrophoresis.
Acknowledgments
The authors are grateful for the technical assistance provided by Dete Hasse, Matthew Kerr, and Peter Walker. This research was funded by the Department of Primary Industries Victoria, The Australian Sheep Industry Cooperative Research Centre, and Meat and Livestock Australia. Antony Bacic acknowledges support received from the Victorian State government STII funding to the Victorian Centre for Plant Functional Genomics. Kris Ferguson is supported by funding from the ARC and GRDC to the Australian Centre for Plant Functional Genomics. The authors thank Dr V. H. Oddy for his constructive comment and critical review of this manuscript.
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