TY - JOUR
T1 - Alternative S2 Hinge Regions of the Myosin Rod Differentially Affect Muscle Function, Myofibril Dimensions and Myosin Tail Length
AU - Suggs, Jennifer A.
AU - Cammarato, Anthony
AU - Kronert, William A.
AU - Nikkhoy, Massoud
AU - Dambacher, Corey M.
AU - Megighian, Aram
AU - Bernstein, Sanford I.
N1 - Funding Information:
We are grateful to Mr Allen Church and Dr Michelle Mardahl-Dumesnil for their technical expertise, and to Mr Gregory Aselis for initial work on the project. We thank Dr Jim Vigoreaux (University of Vermont) and Dr Sunita Patel (Brigham and Women's Hospital) for unpublished data and Dr Venky Iyer (University of California, Berkeley) for Drosophila Mhc gene alignments. We appreciate the advice of Dr Roger Craig (University of Massachusetts Medical School) and Dr Steve Barlow regarding sample preparation and electron microscopy. We thank Dr Douglas Deutschman for consultation on statistical analysis. We appreciate the helpful discussions and manuscript review provided by D. Douglas Swank (Rensselaer Polytechnic Institute), Dr Jim Vigoreaux, Dr Mark Miller (University of Vermont), Dr David Maughan (University of Vermont), Dr Yudong Hao (University of Washington), Dr Gerald Pollack (University of Washington) and Dr Aileen Knowles. This work was supported by grant R01-AR43396 to S.I.B. from the NIH/ National Institute of Arthritis and Musculoskeletal Disease and a postdoctoral research supplement from NIH to A.C.
PY - 2007/4/13
Y1 - 2007/4/13
N2 - Muscle myosin heavy chain (MHC) rod domains intertwine to form alpha-helical coiled-coil dimers; these subsequently multimerize into thick filaments via electrostatic interactions. The subfragment 2/light meromyosin "hinge" region of the MHC rod, located in the C-terminal third of heavy meromyosin, may form a less stable coiled-coil than flanking regions. Partial "melting" of this region has been proposed to result in a helix to random-coil transition. A portion of the Drosophila melanogaster MHC hinge is encoded by mutually exclusive alternative exons 15a and 15b, the use of which correlates with fast (hinge A) or slow (hinge B) muscle physiological properties. To test the functional significance of alternative hinge regions, we constructed transgenic fly lines in which fast muscle isovariant hinge A was switched for slow muscle hinge B in the MHC isoforms of indirect flight and jump muscles. Substitution of the slow muscle hinge B impaired flight ability, increased sarcomere lengths by approximately 13% and resulted in minor disruption to indirect flight muscle sarcomeric structure compared with a transgenic control. With age, residual flight ability decreased rapidly and myofibrils developed peripheral defects. Computational analysis indicates that hinge B has a greater coiled-coil propensity and thus reduced flexibility compared to hinge A. Intriguingly, the MHC rod with hinge B was ∼5 nm longer than myosin with hinge A, consistent with the more rigid coiled-coil conformation predicted for hinge B. Our study demonstrates that hinge B cannot functionally substitute for hinge A in fast muscle types, likely as a result of differences in the molecular structure of the rod, subtle changes in myofibril structure and decreased ability to maintain sarcomere structure in indirect flight muscle myofibrils. Thus, alternative hinges are important in dictating the distinct functional properties of myosin isoforms and the muscles in which they are expressed.
AB - Muscle myosin heavy chain (MHC) rod domains intertwine to form alpha-helical coiled-coil dimers; these subsequently multimerize into thick filaments via electrostatic interactions. The subfragment 2/light meromyosin "hinge" region of the MHC rod, located in the C-terminal third of heavy meromyosin, may form a less stable coiled-coil than flanking regions. Partial "melting" of this region has been proposed to result in a helix to random-coil transition. A portion of the Drosophila melanogaster MHC hinge is encoded by mutually exclusive alternative exons 15a and 15b, the use of which correlates with fast (hinge A) or slow (hinge B) muscle physiological properties. To test the functional significance of alternative hinge regions, we constructed transgenic fly lines in which fast muscle isovariant hinge A was switched for slow muscle hinge B in the MHC isoforms of indirect flight and jump muscles. Substitution of the slow muscle hinge B impaired flight ability, increased sarcomere lengths by approximately 13% and resulted in minor disruption to indirect flight muscle sarcomeric structure compared with a transgenic control. With age, residual flight ability decreased rapidly and myofibrils developed peripheral defects. Computational analysis indicates that hinge B has a greater coiled-coil propensity and thus reduced flexibility compared to hinge A. Intriguingly, the MHC rod with hinge B was ∼5 nm longer than myosin with hinge A, consistent with the more rigid coiled-coil conformation predicted for hinge B. Our study demonstrates that hinge B cannot functionally substitute for hinge A in fast muscle types, likely as a result of differences in the molecular structure of the rod, subtle changes in myofibril structure and decreased ability to maintain sarcomere structure in indirect flight muscle myofibrils. Thus, alternative hinges are important in dictating the distinct functional properties of myosin isoforms and the muscles in which they are expressed.
KW - Drosophila
KW - S2 hinge
KW - indirect flight muscle
KW - myofibril
KW - myosin
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U2 - 10.1016/j.jmb.2007.01.045
DO - 10.1016/j.jmb.2007.01.045
M3 - Article
C2 - 17316684
AN - SCOPUS:33947150032
SN - 0022-2836
VL - 367
SP - 1312
EP - 1329
JO - Journal of molecular biology
JF - Journal of molecular biology
IS - 5
ER -