Abstract

The aim of these studies is to understand in detail the structure of two kinds of filaments in striated muscle--the myosin-containing, thick filaments and the desmin-containing intermediate filaments. The filaments will be studied at three levels of structural organization--the subunits of assembly, the filaments themselves and, in the case of thick filaments, the filament lattice. A unique morphological approach--quick-freezing followed by freeze-etching and rotary replication--will be used to prepare samples for electron microscopy. To study thick filament and crossbridge structure, intact muscle fibers as well as fractionated thin filaments with an """"""""in vivo"""""""" complement of crossbridges will be quick-frozen, examined by electron microscopy and analyzed by image processing techniques. The location of the light chains in the myosin molecule will also be determined morphologically and verified using monoclonal antibodies directed against light chain epitopes. The assembly of intermediate filaments from their building blocks (protofilaments) will be studied using in vitro systems. The effects of two monoclonal antibodies to desmin, known to bind to protofilament ends, upon the polymerization of desmin will be assessed quantitatively as well as by electron microscopy. The possible existence of assembly intermediates will be probed by assembling purified vimentin protofilaments at sub-physiological salt concentrations, isolating the intermediate species and testing their ability to modulate further IF polymerization. Rate constants and directionality of polymerization will be determined. Information obtained in these studies will help to understand the molecular events during muscular contraction, and how muscle contraction is coordinated at the level of the cytoskeleton. The elucidation of muscle intermediate filament structure will also likely be of general applicability to other subclasses of filaments in epithelial cells and cells of the nervous system, since all intermediate filament proteins are now known to share homologous amino acid sequences.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Arthritis and Musculoskeletal and Skin Diseases (NIAMS)
Type
Research Project (R01)
Project #
5R01AR035973-02
Application #
3157425
Study Section
Cellular Biology and Physiology Subcommittee 1 (CBY)
Project Start
1985-01-01
Project End
1987-12-31
Budget Start
1986-01-01
Budget End
1986-12-31
Support Year
2
Fiscal Year
1986
Total Cost
Indirect Cost

  Institution

Name
University of Cincinnati
Department
Type
Schools of Medicine
DUNS #
City
Cincinnati
State
OH
Country
United States
Zip Code
45221

  Publications

Meng, J J; Ip, W (2001) A yeast two-hybrid approach for probing cytoskeletal protein interactions. Methods Mol Biol 161:255-68
Meng, J J; Bornslaeger, E A; Green, K J et al. (1997) Two-hybrid analysis reveals fundamental differences in direct interactions between desmoplakin and cell type-specific intermediate filaments. J Biol Chem 272:21495-503
Carpenter, D A; Ip, W (1996) Neurofilament triplet protein interactions: evidence for the preferred formation of NF-L-containing dimers and a putative function for the end domains. J Cell Sci 109 ( Pt 10):2493-8
Meng, J J; Khan, S; Ip, W (1996) Intermediate filament protein domain interactions as revealed by two-hybrid screens. J Biol Chem 271:1599-604
Meng, J J; Khan, S; Ip, W (1994) Charge interactions in the rod domain drive formation of tetramers during intermediate filament assembly. J Biol Chem 269:18679-85
Makarova, I; Carpenter, D; Khan, S et al. (1994) A conserved region in the tail domain of vimentin is involved in its assembly into intermediate filaments. Cell Motil Cytoskeleton 28:265-77
Mulligan, L; Balin, B J; Lee, V M et al. (1991) Antibody labeling of bovine neurofilaments: implications on the structure of neurofilament sidearms. J Struct Biol 106:145-60
Tao, J X; Ip, W (1991) Site-specific antibodies block kinase A phosphorylation of desmin in vitro and inhibit incorporation of myoblasts into myotubes. Cell Motil Cytoskeleton 19:109-20
Birkenberger, L; Ip, W (1990) Properties of the desmin tail domain: studies using synthetic peptides and antipeptide antibodies. J Cell Biol 111:2063-75
Ip, W; Saeed, T (1990) Desmin-binding specificities of two desmin CNBr fragments that correspond to the headpiece domain and Helix 1B. Cell Biol Int Rep 14:1119-27

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