Lysine acetylation of F-actin decreases tropomyosin-based inhibition of actomyosin activity

William Schmidt; Aditi Madan; D Brian Foster; Anthony Cammarato

doi:10.1074/jbc.RA120.015277

Lysine acetylation of F-actin decreases tropomyosin-based inhibition of actomyosin activity

J Biol Chem. 2020 Nov 13;295(46):15527-15539. doi: 10.1074/jbc.RA120.015277. Epub 2020 Sep 1.

Authors

William Schmidt¹, Aditi Madan¹, D Brian Foster¹, Anthony Cammarato²

Affiliations

¹ Department of Medicine, Johns Hopkins University School of Medicine, Baltimore, Maryland, USA.
² Department of Medicine, Johns Hopkins University School of Medicine, Baltimore, Maryland, USA. Electronic address: acammar3@jhmi.edu.

Abstract

Recent proteomics studies of vertebrate striated muscle have identified lysine acetylation at several sites on actin. Acetylation is a reversible post-translational modification that neutralizes lysine's positive charge. Positively charged residues on actin, particularly Lys³²⁶ and Lys³²⁸, are predicted to form critical electrostatic interactions with tropomyosin (Tpm) that promote its binding to filamentous (F)-actin and bias Tpm to an azimuthal location where it impedes myosin attachment. The troponin (Tn) complex also influences Tpm's position along F-actin as a function of Ca²⁺ to regulate exposure of myosin-binding sites and, thus, myosin cross-bridge recruitment and force production. Interestingly, Lys³²⁶ and Lys³²⁸ are among the documented acetylated residues. Using an acetic anhydride-based labeling approach, we showed that excessive, nonspecific actin acetylation did not disrupt characteristic F-actin-Tpm binding. However, it significantly reduced Tpm-mediated inhibition of myosin attachment, as reflected by increased F-actin-Tpm motility that persisted in the presence of Tn and submaximal Ca²⁺ Furthermore, decreasing the extent of chemical acetylation, to presumptively target highly reactive Lys³²⁶ and Lys³²⁸, also resulted in less inhibited F-actin-Tpm, implying that modifying only these residues influences Tpm's location and, potentially, thin filament regulation. To unequivocally determine the residue-specific consequences of acetylation on Tn-Tpm-based regulation of actomyosin activity, we assessed the effects of K326Q and K328Q acetyl (Ac)-mimetic actin on Ca²⁺-dependent, in vitro motility parameters of reconstituted thin filaments (RTFs). Incorporation of K328Q actin significantly enhanced Ca²⁺ sensitivity of RTF activation relative to control. Together, our findings suggest that actin acetylation, especially Lys³²⁸, modulates muscle contraction via disrupting inhibitory Tpm positioning.

Keywords: acetylation; actin; in vitro motility; lysine acetylation; muscle physiology; myosin; thin filament; tropomyosin.

Publication types

Research Support, N.I.H., Extramural
Research Support, Non-U.S. Gov't

MeSH terms

Acetylation
Actins / chemistry
Actins / genetics
Actins / metabolism*
Actomyosin / antagonists & inhibitors
Actomyosin / metabolism*
Amino Acid Sequence
Animals
Animals, Genetically Modified / metabolism
Binding Sites
Calcium / metabolism
Cattle
Drosophila / metabolism
Drosophila Proteins / chemistry
Drosophila Proteins / genetics
Drosophila Proteins / metabolism
Kinetics
Lysine / metabolism
Molecular Dynamics Simulation
Mutagenesis, Site-Directed
Protein Binding
Rabbits
Swine
Tropomyosin / metabolism*

Substances

Actins
Drosophila Proteins
Tropomyosin
Actomyosin
Lysine
Calcium

Associated data

PDB/4A7f
PDB/9PDB

Abstract

Publication types

MeSH terms

Substances

Associated data

Grants and funding