Your search keyword '"Hennessey E"' showing total 10 results

1. Actomyosin kinetics and in vitro motility of wild-type Drosophila actin and the effects of two mutations in the Act88F gene.

Author

Anson M, Drummond DR, Geeves MA, Hennessey ES, Ritchie MD, and Sparrow JC

Subjects

Actins genetics, Adenosine Diphosphate metabolism, Adenosine Triphosphatases metabolism, Adenosine Triphosphate metabolism, Amino Acid Sequence, Animals, Drosophila genetics, Homozygote, Kinetics, Models, Molecular, Rabbits, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Actins chemistry, Actins metabolism, Actomyosin chemistry, Actomyosin metabolism, Drosophila metabolism, Point Mutation, Protein Structure, Secondary

Abstract

Two missense mutations of the flight muscle-specific actin gene of Drosophila melanogaster, Act88F, assemble into normally structured myofibrils but affect the flight ability of flies and the mechanical kinetics of isolated muscle fibers. We describe the isolation of actin from different homozygous Act88F strains, including wild-type, an Act88F null mutant (KM88), and two Act88F single point mutations (E316K and G368E), their biochemical interactions with rabbit myosin subfragment 1 (S1), and behavior with rabbit myosin and heavy meromyosin in in vitro motility assays. The rabbit and wild-type Drosophila actins have different association rate constants with S1 (2.64 and 1.77 microM-1 s-1, respectively) and in vitro motilities (2.51, 1.60 microns s-1) clearly demonstrating an isoform-specific difference. The G368E mutation shows a reduced affinity for rabbit S1 compared with the wild type (increasing from 0.11 to 0.17 microM) and a reduced velocity in vitro (reduced by 19%). The E316K mutant actin has no change in affinity for myosin S1 or in vitro motility with heavy meromyosin but does have a reduced in vitro motility (15%) with myosin. These results are discussed with respect to the recently published atomic models for the actomyosin structure and our findings that G368E fibers show a reduced rate constant for delayed tension development and increased fiber stiffness. We interpret these results as possibly caused either by effects on A1 myosin light chain binding or conformational changes within the subdomain 1 of actin, which contains the myosin binding site. E316K is discussed with respect to its likely position within the tropomyosin binding site of actin.

Published

1995

2. Molecular genetics of actin function.

Author

Hennessey ES, Drummond DR, and Sparrow JC

Subjects

Amino Acid Sequence, Animals, Conserved Sequence, Humans, Models, Molecular, Molecular Structure, Muscles chemistry, Muscles physiology, Mutagenesis, Actins genetics, Actins physiology

Published

1993

3. ADP-ribosylation of Drosophila indirect-flight-muscle actin and arthrin by Clostridium botulinum C2 toxin and Clostridium perfringens iota toxin.

Author

Just I, Hennessey ES, Drummond DR, Aktories K, and Sparrow JC

Subjects

Actins genetics, Animals, Arginine metabolism, Botulinum Toxins metabolism, Clostridium botulinum, Clostridium perfringens, Drosophila genetics, Enterotoxins metabolism, Flight, Animal, Insect Proteins, Muscles chemistry, Mutagenesis, Rabbits, Transfection, Ubiquitin, ADP Ribose Transferases, Actins metabolism, Adenosine Diphosphate Ribose metabolism, Bacterial Toxins metabolism, Drosophila chemistry, Microfilament Proteins metabolism, Muscle Proteins metabolism, Toxoids metabolism

Abstract

Purified Drosophila indirect-flight-muscle actin and arthrin, an actin-ubiquitin conjugate, were ADP-ribosylated by Clostridium botulinum C2 toxin and Clostridium perfringens iota toxin. Phalloidin treatment inhibited the ADP-ribosylation of Drosophila actin and arthrin. Like actin, the ADP-ribose-arthrin linkage was sensitive towards hydroxylamine treatment, indicating arginine as the amino acid acceptor. Actin translated in vitro from the indirect-flight-muscle-specific gene Act88F was ADP-ribosylated by C. botulinum C2 toxin and C. perfringens iota toxin. Actin from the R177Q mutant of Act88F translated in vivo was not ADP-ribosylated confirming Arg-177 as the ADP-ribose acceptor. Mutant L176M actin was modified by both toxins, indicating that amino acid 176 of actin does not define the substrate specificity of C. botulinum C2 toxin. Whereas the gene products of various C-terminal mutants of Act88F translated in vitro (E334K, V339I, E364K, G368E, R372H) were substrates for ADP-ribosylation by C. botulinum C2 toxin and by C. perfringens iota toxin, neither toxin modified the N-terminal O-12 deletion mutant.

Published

1993

4. The binding of mutant actins to profilin, ATP and DNase I.

Author

Drummond DR, Hennessey ES, and Sparrow JC

Subjects

Actins chemistry, Actins genetics, Amino Acid Sequence, Animals, Drosophila Proteins, Electrophoresis, Polyacrylamide Gel, Kinetics, Profilins, Protein Binding, Protein Conformation, Structure-Activity Relationship, Actins metabolism, Adenosine Triphosphate metabolism, Contractile Proteins, Deoxyribonuclease I metabolism, Drosophila melanogaster genetics, Microfilament Proteins metabolism, Mutagenesis

Abstract

Twenty-five mutations were created in the Drosophila melanogaster Act88F actin gene by in vitro mutagenesis and the mutant actins expressed in vitro. The affinity of the mutant actins for ATP, profilin and DNase I was determined. They were also tested for conformational changes by non-denaturing gel electrophoresis. Mutations at positions 364 (highly conserved) and 366 (invariant) caused changes in conformation, reduced ATP binding and increased profilin binding. At position 362 (invariant) only the conservative change from tyrosine to phenylalanine had no effect; other changes at this position affected conformation, ATP and profilin binding. Although only glycine or serine occur naturally at position 368, changes to threonine or glutamine had no effect on the actin. The mutant in which Asp363 was replaced by His and that in which Glu364 was replaced by Lys decreased DNase I binding, yet neither amino acid occurs in the DNase I binding site. Likewise several mutations affect ATP and profilin binding but are distant from the binding sites. We conclude that, although actin has a highly conserved amino acid sequence, individual amino acids can have variable tolerance for substitutions. Also amino acid changes can exert significant effects on the binding of ligands to distant parts of the actin structure.

Published

1992

5. Mutant actin: a dead end?

Author

Hennessey ES, Harrison A, Drummond DR, and Sparrow JC

Subjects

Actin Cytoskeleton metabolism, Actins metabolism, Actins ultrastructure, Animals, Cell-Free System, Drosophila melanogaster genetics, Escherichia coli, Genes, Lethal, Polymers, Protein Biosynthesis, Protein Engineering, Rabbits, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Reticulocytes metabolism, Saccharomyces cerevisiae, Structure-Activity Relationship, Actins genetics

Published

1992

6. Drosophila actin mutants and the study of myofibrillar assembly and function.

Author

Sparrow JC, Drummond DR, Hennessey ES, Clayton JD, and Lindegaard FB

Subjects

Actins chemistry, Actins metabolism, Animals, Drosophila genetics, Macromolecular Substances, Microscopy, Electron, Muscles ultrastructure, Mutation, Protein Processing, Post-Translational physiology, Structure-Activity Relationship, Actins genetics, Muscles chemistry

Abstract

The use of Drosophila mutations in the indirect flight muscle-specific actin gene, Act88F, to study actin structure/function and its assembly into thin filaments during myofibrillogenesis is described. Mutants with different phenotypic effects are discussed and attempts made to correlate the different properties of the mutants in vivo-myofibrillar structure, actin synthesis, accumulation and stability, heat shock response induction-with properties of the same mutations expressed by in vitro transcription/translation of the cloned actin genes-co-polymerisation, thermostability and protein conformation. Few of the properties show a complete correlation between the different classes of mutants. The nature of the diversity of the mutant effects is discussed. Questions as to how this will help in elucidating the molecular effects of the mutations and the assembly of thin filaments and myofibrils are considered. In addition, the efficacy of the co-polymerisation assay is examined. The post-translational processing of this actin-by N-terminal processing, methylation and ubiquitination-are described. Data is presented that inhibition of the N-terminal processing of actin in vitro affects the ability of the actin to copolymerise, and makes unprocessed actin behave as a capping protein. The possible in vivo importance of this phenomenon is discussed.

Published

1992

7. Functional and ultrastructural effects of a missense mutation in the indirect flight muscle-specific actin gene of Drosophila melanogaster.

Author

Sparrow J, Reedy M, Ball E, Kyrtatas V, Molloy J, Durston J, Hennessey E, and White D

Subjects

Actins isolation & purification, Amino Acid Sequence, Animals, Cloning, Molecular, Drosophila melanogaster physiology, Flight, Animal, Glutamates, Glutamic Acid, Lysine, Microscopy, Electron, Muscle Proteins isolation & purification, Muscle Relaxation, Muscles physiology, Myofibrils ultrastructure, Peptide Mapping, Actins genetics, Drosophila melanogaster genetics, Muscles ultrastructure, Mutation

Abstract

A single-site mutation of the flight-muscle-specific actin gene of Drosophila melanogaster causes a substitution of glutamic acid 93 by lysine in all the actin encoded in the indirect flight muscle (IFM). In these Act88FE93K mutants, myofibrillar bundles of thick and thin filaments are present but lack Z-discs and all sarcomeric repeats. Dense filament bundles, which are probably aberrant Z-discs, are seen in myofibrils of pupal flies, but early in adult life these move to the periphery of the fibrils and are not seen in skinned adult fibres. Consistent with this observation, alpha-actinin and other high molecular weight proteins, possibly associated with Z-discs, are not detected on SDS/polyacrylamide gels or Western blots of skinned adult IFM. The mutation lies at the beginning of a loop in the small domain of actin, near the myosin binding region. However, that the mutant actin binds myosin heads is shown by (1) rigor crossbridges in electron micrographs, (2) the appropriate rise in stiffness when ATP is withdrawn in mechanical experiments, and (3) equal protection against tryptic digestion provided by rigor binding between actin and myosin in both wild-type and mutant fibres. Reversal of rigor chevron angle along some thin filaments reflects reversal of thin-filament polarity due to lattice disorder. The absence of Z-discs, alpha-actinin and two high molecular weight proteins, and binding studies by others, suggest that the substitution at residue 93 affects the binding of the mutant actin to a protein, possibly alpha-actinin, which is necessary for Z-disc assembly or maintenance.

Published

1991

8. Post-translational processing of the amino terminus affects actin function.

Author

Hennessey ES, Drummond DR, and Sparrow JC

Subjects

Animals, Electrophoresis, Gel, Two-Dimensional, Peptide Mapping, Polymers, Protein Biosynthesis, Rabbits, Transcription, Genetic, Actins physiology, Drosophila melanogaster genetics, Protein Processing, Post-Translational

Abstract

We have studied the importance of N-terminal processing for normal actin function using the Drosophila Act88F actin gene transcribed and translated in vitro. Despite having different charges as determined by two-dimensional (2D) gel electrophoresis, Act88F expressed in vivo and in vitro in rabbit reticulocyte lysate bind to DNase I with equal affinity and are able to copolymerise with bulk rabbit actin equally well. Using peptide mapping and thin-layer electrophoresis we have shown that bestatin [( 3-amino-2-hydroxy-4-phenyl-butanoyl]-L-leucine), an inhibitor of aminopeptidases, can inhibit actin N-terminal processing in rabbit reticulocyte lysate. Although processed and unprocessed actins translated in vitro are able to bind to DNase I equally well, unprocessed actins are less able to copolymerise with bulk actins. This effect is more pronounced when bulk rabbit actin is used but is still seen with bulk Lethocerus actin. Also, the unprocessed actins reduce the polymerisation of the processed actin translated in vitro with the bulk rabbit actin. This suggests that individual actins do interact, even in non-polymerising conditions. The reduced ability of unprocessed actin to polymerise shows that correct post-translational modification of the N terminus is required for normal actin function.

Published

1991

9. Characterisation of missense mutations in the Act88F gene of Drosophila melanogaster.

Author

Drummond DR, Hennessey ES, and Sparrow JC

Subjects

Actins metabolism, Animals, Cloning, Molecular, DNA Transposable Elements, Electrophoresis, Gel, Two-Dimensional, Heat-Shock Proteins metabolism, Molecular Conformation, Muscles cytology, Muscles ultrastructure, Mutagenesis, Myosins metabolism, Phenotype, Polymers, Transformation, Genetic, Actins genetics, Drosophila melanogaster genetics, Mutation genetics

Abstract

We have created missense mutations in the indirect flight muscle (IFM)-specific Act88F actin gene of Drosophila melanogaster by random in vitro mutagenesis. Following P element-mediated transformation into wild-type flies and subsequent transfer of the inserts into Act88F null strains, the effects of the actin mutants on the structure and function of the IFMs were examined. All of the mutants were antimorphic for flight ability. E316K and G368E formed muscle with only relatively small defects in structure whilst the others produced IFMs with large amounts of disruption. E334K formed filaments but lacked Z discs. V339I formed no muscle structure in null flies and did not accumulate actin. E364K and G366D both had relatively stable actin but did not form myofibrils. Using an in vitro polymerisation assay we found no significant effects on the ability of the mutant actins to polymerise. E364K and G366D also caused a strong induction of heat shock protein (hsp) synthesis at normal temperatures and accumulated large amounts of hsp22 which, together with the mutant actin, was resistant to detergent extraction. Both E316K and E334K caused a weak induction of hsp synthesis. We discuss how the stability, structure and function of the different mutant actins affects myofibril assembly and function, and the induction of hsps.

Published

1991

10. Stability of mutant actins.

Author

Drummond DR, Hennessey ES, and Sparrow JC

Subjects

Actins genetics, Animals, Drosophila, Drug Stability, Electrophoresis, Polyacrylamide Gel, Mutation, Protein Biosynthesis, Protein Denaturation, Rabbits, Transcription, Genetic, Urea, Actins chemistry

Abstract

Mutants of the Drosophila Act88F actin gene were transcribed and translated in vitro and their relative stabilities were examined using urea gradient gel electrophoresis. Most of the mutant actins (E334K, E364K, G366D, G368E and R372H) were as stable as the wild-type. V339I had a slight decrease in stability, and E316K was the least stable. The causes of the differences are discussed and contrasted with the behaviour of the mutants in vivo, where E316K has normal stability and V339I is the least stable.

Published

1991