The primary cause of muscle disfunction associated with substitutions E240K and R244G in tropomyosin is aberrant behavior of tropomyosin and response of actin and myosin during ATPase cycle

Armen O Simonyan; Vladimir V Sirenko; Olga E Karpicheva; Katarzyna Robaszkiewicz; Małgorzata Śliwinska; Joanna Moraczewska; Zoya I Krutetskaya; Yurii S Borovikov

doi:10.1016/j.abb.2018.03.002

The primary cause of muscle disfunction associated with substitutions E240K and R244G in tropomyosin is aberrant behavior of tropomyosin and response of actin and myosin during ATPase cycle

Arch Biochem Biophys. 2018 Apr 15:644:17-28. doi: 10.1016/j.abb.2018.03.002. Epub 2018 Mar 3.

Authors

Armen O Simonyan¹, Vladimir V Sirenko², Olga E Karpicheva², Katarzyna Robaszkiewicz³, Małgorzata Śliwinska³, Joanna Moraczewska³, Zoya I Krutetskaya⁴, Yurii S Borovikov⁵

Affiliations

¹ Institute of Cytology of the Russian Academy of Sciences, Laboratory of Molecular Basis of Cell Motility, 4 Tikhoretsky Ave., 194064, Saint Petersburg, Russia; Saint Petersburg State University, Faculty of Biology, Department of Biophysics, 7/9 Universitetskaya Emb., 199034, Saint Petersburg, Russia.
² Institute of Cytology of the Russian Academy of Sciences, Laboratory of Molecular Basis of Cell Motility, 4 Tikhoretsky Ave., 194064, Saint Petersburg, Russia.
³ Kazimierz Wielki University in Bydgoszcz, Institute of Experimental Biology, Department of Biochemistry and Cell Biology, Ks. J. Poniatowski 12 Str., 85-671, Bydgoszcz, Poland.
⁴ Saint Petersburg State University, Faculty of Biology, Department of Biophysics, 7/9 Universitetskaya Emb., 199034, Saint Petersburg, Russia.
⁵ Institute of Cytology of the Russian Academy of Sciences, Laboratory of Molecular Basis of Cell Motility, 4 Tikhoretsky Ave., 194064, Saint Petersburg, Russia. Electronic address: borovikov@incras.ru.

PMID: 29510086
DOI: 10.1016/j.abb.2018.03.002

Abstract

Using the polarized photometry technique we have studied the effects of two amino acid replacements, E240K and R244G, in tropomyosin (Tpm1.1) on the position of Tpm1.1 on troponin-free actin filaments and the spatial arrangement of actin monomers and myosin heads at various mimicked stages of the ATPase cycle in the ghost muscle fibres. E240 and R244 are located in the C-terminal, seventh actin-binding period, in f and b positions of the coiled-coil heptapeptide repeat. Actin, Tpm1.1, and myosin subfragment-1 (S1) were fluorescently labeled: 1.5-IAEDANS was attached to actin and S1, 5-IAF was bound to Tpm1.1. The labeled proteins were incorporated in the ghost muscle fibres and changes in polarized fluorescence during the ATPase cycle have been measured. It was found that during the ATPase cycle both mutant tropomyosins occupied a position close to the inner domain of actin. The relative amount of the myosin heads in the strongly-bound conformations and of the switched on actin monomers increased at mimicking different stages of the ATPase cycle. This might be one of the reasons for muscle dysfunction in congenital fibre type disproportion caused by the substitutions E240K and R244G in tropomyosin.

Keywords: Congenital myopathies; F-actin; Fluorescence polarization; Ghost muscle fibres; Myosin; Tropomyosin; Troponin.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Actins / chemistry*
Actins / genetics
Actins / metabolism
Amino Acid Substitution
Humans
Muscle Fibers, Skeletal / chemistry*
Muscle Fibers, Skeletal / metabolism
Muscle Fibers, Skeletal / pathology
Muscular Diseases / genetics
Muscular Diseases / metabolism
Muscular Diseases / pathology
Mutation, Missense*
Myosins / chemistry*
Myosins / genetics
Myosins / metabolism
Tropomyosin / chemistry*
Tropomyosin / genetics
Tropomyosin / metabolism

Substances

Actins
Tropomyosin
Myosins