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1. Mechanoregulated inhibition of formin facilitates contractile actomyosin ring assembly

Author

Dennis Zimmermann, Kaitlin E. Homa, Glen M. Hocky, Luther W. Pollard, Enrique M. De La Cruz, Gregory A. Voth, Kathleen M. Trybus, and David R. Kovar

Subjects
Science
Abstract

The fission yeast cytokinetic ring assembles by Search-Capture-Pull-Release from precursor nodes that include formin Cdc12 and myosin Myo2. The authors reconstitute Search-Capture-Pull in vitro and find that Myo2 pulling on Cdc12-associated actin filaments mechano-inhibits Cdc12-mediated assembly, which enables proper ring assembly in vivo.

Published
2017
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2. Acetylation of fission yeast tropomyosin does not promote differential association with cognate formins

Author

Qing Tang, Luther W. Pollard, Kaitlin E. Homa, David R. Kovar, and Kathleen M. Trybus

Subjects
Structural Biology, Cell Biology
Abstract

It was proposed from cellular studies thatS. pombetropomyosin Cdc8 (Tpm) segregates into two populations due to the presence or absence of an amino-terminal acetylation that specifies which formin-mediated F-actin networks it binds, but with no supporting biochemistry. To address this mechanismin vitro, we developed methods forS. pombeactin expression in Sf9 cells. We then employed 3-color TIRF microscopy using all recombinantS. pombeproteins to probein vitromulticomponent mechanisms involving actin, acetylated and unacetylated Tpm, formins, and myosins. Acetyl-Tpm exhibits tight binding to actin in contrast to weaker binding by unacetylated Tpm. In disagreement with the differential recruitment model, Tpm showed no preferential binding to filaments assembled by the FH1-FH2-domains of twoS. pombeformins, nor did Tpm binding have any bias towards the growing formin-bound actin filament barbed end. Although ourin vitrofindings do not support a direct formin-tropomyosin interaction, it is possible that formins bias differential tropomyosin isoform recruitment through undiscovered mechanisms. Importantly, despite a 12% sequence divergence between skeletal andS. pombeactin,S. pombemyosins Myo2 and Myo51 exhibited similar motile behavior with these two actins, validating key prior findings with these myosins that used skeletal actin.

Published
2022
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3. Genetically inspired in vitro reconstitution ofSaccharomyces cerevisiaeactin cables from seven purified proteins

Author

Mikael V. Garabedian, Bruce L. Goode, Luther W. Pollard, Salvatore L. Alioto, and Shashank Shekhar

Subjects
biology, Biochemistry, Saccharomyces cerevisiae, Cell Biology, biology.organism_classification, Molecular Biology, Actin, Yeast, In vitro
Abstract

Yeast actin cables are reconstituted from seven purified proteins, providing a powerful demonstration of how a minimal set of components can self-organize into a micron-scale structure that has many of the same features of actin cables found in vivo.

Published
2020
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6. WAVE1 and WAVE2 have distinct and overlapping roles in controlling actin assembly at the leading edge

Author

Bruce L. Goode, Changsong Yang, Klemens Rottner, Qing Tang, Tatyana Svitkina, Neha Koundinya, Matthias Schaks, Luther W. Pollard, and HZI,Helmholtz-Zentrum für Infektionsforschung GmbH, Inhoffenstr. 7,38124 Braunschweig, Germany.

Subjects
Gene isoform, Leading edge, Cell, Motility, macromolecular substances, Biology, Actin-Related Protein 2-3 Complex, Protein filament, Cell Movement, Cell Line, Tumor, medicine, Humans, Pseudopodia, Molecular Biology, Actin, Actin nucleation, Microfilament Proteins, Cell Biology, Actins, Cell biology, Wiskott-Aldrich Syndrome Protein Family, Actin Cytoskeleton, medicine.anatomical_structure, Brief Reports, Cell Surface Extensions, Lamellipodium
Abstract

SCAR/WAVE proteins and Arp2/3 complex assemble branched actin networks at the leading edge. Two isoforms of SCAR/WAVE, WAVE1 and WAVE2, reside at the leading edge, yet it has remained unclear whether they perform similar or distinct roles. Further, there have been conflicting reports about the Arp2/3-independent biochemical activities of WAVE1 on actin filament elongation. To investigate this in vivo, we knocked out WAVE1 and WAVE2 genes, individually and together, in B16-F1 melanoma cells. We demonstrate that WAVE1 and WAVE2 are redundant for lamellipodia formation and motility. However, there is a significant decrease in the rate of leading edge actin extension in WAVE2 KO cells, and an increase in WAVE1 KO cells. The faster rates of actin extension in WAVE1 KO cells are offset by faster retrograde flow, and therefore do not translate into faster lamellipodium protrusion. Thus, WAVE1 restricts the rate of actin extension at the leading edge, and appears to couple actin networks to the membrane to drive protrusion. Overall, these results suggest that WAVE1 and WAVE2 have redundant roles in promoting Arp2/3-dependent actin nucleation and lamellipodia formation, but distinct roles in controlling actin network extension and harnessing network growth to cell protrusion.

Published
2020

7. UCS protein Rng3p is essential for myosin-II motor activity during cytokinesis in fission yeast.

Author

Benjamin C Stark, Michael L James, Luther W Pollard, Vladimir Sirotkin, and Matthew Lord

Subjects
Medicine, Science
Abstract

UCS proteins have been proposed to operate as co-chaperones that work with Hsp90 in the de novo folding of myosin motors. The fission yeast UCS protein Rng3p is essential for actomyosin ring assembly and cytokinesis. Here we investigated the role of Rng3p in fission yeast myosin-II (Myo2p) motor activity. Myo2p isolated from an arrested rng3-65 mutant was capable of binding actin, yet lacked stability and activity based on its expression levels and inactivity in ATPase and actin filament gliding assays. Myo2p isolated from a myo2-E1 mutant (a mutant hyper-sensitive to perturbation of Rng3p function) showed similar behavior in the same assays and exhibited an altered motor conformation based on limited proteolysis experiments. We propose that Rng3p is not required for the folding of motors per se, but instead works to ensure the activity of intrinsically unstable myosin-II motors. Rng3p is specific to conventional myosin-II and the actomyosin ring, and is not required for unconventional myosin motor function at other actin structures. However, artificial destabilization of myosin-I motors at endocytic actin patches (using a myo1-E1 mutant) led to recruitment of Rng3p to patches. Thus, while Rng3p is specific to myosin-II, UCS proteins are adaptable and can respond to changes in the stability of other myosin motors.

Published
2013
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8. Integrated control of formin-mediated actin assembly by a stationary inhibitor and a mobile activator

Author

Olga Sokolova, Bruce L. Goode, Chenyu Lou, Thomas J. Rands, Luther W. Pollard, Mikael V. Garabedian, and T.B. Stanishneva-Konovalova

Subjects
0301 basic medicine, Saccharomyces cerevisiae Proteins, Saccharomyces cerevisiae, macromolecular substances, Article, 03 medical and health sciences, Protein Domains, In vivo, Animals, Actin, Research Articles, Actin nucleation, biology, Activator (genetics), Secretory Vesicles, Microfilament Proteins, Cell Biology, biology.organism_classification, Secretory Vesicle, In vitro, Actins, Cell biology, Cytoskeletal Proteins, 030104 developmental biology, Formins, biology.protein, Rabbits, Protein Multimerization, Microtubule-Associated Proteins
Abstract

This study shows that in vivo actin nucleation by the yeast formin Bnr1 is controlled through the coordinated effects of two distinct regulators, a stationary inhibitor (the F-BAR protein Hof1) and a mobile activator (Bud6), establishing a positive feedback loop for precise spatial and temporal control of actin assembly., Formins are essential actin assembly factors whose activities are controlled by a diverse array of binding partners. Until now, most formin ligands have been studied on an individual basis, leaving open the question of how multiple inputs are integrated to regulate formins in vivo. Here, we show that the F-BAR domain of Saccharomyces cerevisiae Hof1 interacts with the FH2 domain of the formin Bnr1 and blocks actin nucleation. Electron microscopy of the Hof1–Bnr1 complex reveals a novel dumbbell-shaped structure, with the tips of the F-BAR holding two FH2 dimers apart. Deletion of Hof1’s F-BAR domain in vivo results in disorganized actin cables and secretory defects. The formin-binding protein Bud6 strongly alleviates Hof1 inhibition in vitro, and bud6Δ suppresses hof1Δ defects in vivo. Whereas Hof1 stably resides at the bud neck, we show that Bud6 is delivered to the neck on secretory vesicles. We propose that Hof1 and Bud6 functions are intertwined as a stationary inhibitor and a mobile activator, respectively.

Published
2018

9. Mechanoregulated inhibition of formin facilitates contractile actomyosin ring assembly

Author

Luther W. Pollard, Gregory A. Voth, David R. Kovar, Kaitlin E Homa, Enrique M. De La Cruz, Glen M. Hocky, Kathleen M. Trybus, and Dennis Zimmermann

Subjects
0301 basic medicine, Multidisciplinary, biology, Science, fungi, General Physics and Astronomy, Actin remodeling, General Chemistry, macromolecular substances, Microfilament, Actin cytoskeleton, General Biochemistry, Genetics and Molecular Biology, Cell biology, 03 medical and health sciences, 030104 developmental biology, Formins, Myosin, biology.protein, lcsh:Q, MDia1, lcsh:Science, Cytokinesis, Actin
Abstract

Cytokinesis physically separates dividing cells by forming a contractile actomyosin ring. The fission yeast contractile ring has been proposed to assemble by Search-Capture-Pull-Release from cytokinesis precursor nodes that include the molecular motor type-II myosin Myo2 and the actin assembly factor formin Cdc12. By successfully reconstituting Search-Capture-Pull in vitro, we discovered that formin Cdc12 is a mechanosensor, whereby myosin pulling on formin-bound actin filaments inhibits Cdc12-mediated actin assembly. We mapped Cdc12 mechanoregulation to its formin homology 1 domain, which facilitates delivery of new actin subunits to the elongating actin filament. Quantitative modeling suggests that the pulling force of the myosin propagates through the actin filament, which behaves as an entropic spring, and thereby may stretch the disordered formin homology 1 domain and impede formin-mediated actin filament elongation. Finally, live cell imaging of mechano-insensitive formin mutant cells established that mechanoregulation of formin Cdc12 is required for efficient contractile ring assembly in vivo. The fission yeast cytokinetic ring assembles by Search-Capture-Pull-Release from precursor nodes that include formin Cdc12 and myosin Myo2. The authors reconstitute Search-Capture-Pull in vitro and find that Myo2 pulling on Cdc12-associated actin filaments mechano-inhibits Cdc12-mediated assembly, which enables proper ring assembly in vivo.

Published
2017
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10. Genetically inspired in vitro reconstitution of

Author

Luther W, Pollard, Mikael V, Garabedian, Salvatore L, Alioto, Shashank, Shekhar, and Bruce L, Goode

Subjects
Saccharomyces cerevisiae Proteins, Mutation, Brief Reports, macromolecular substances, Saccharomyces cerevisiae, Actins
Abstract

A major goal of synthetic biology is to define the minimal cellular machinery required to assemble a biological structure in its simplest form. Here, we focused on Saccharomyces cerevisiae actin cables, which provide polarized tracks for intracellular transport and maintain defined lengths while continuously undergoing rapid assembly and turnover. Guided by the genetic requirements for proper cable assembly and dynamics, we show that seven evolutionarily conserved S. cerevisiae proteins (actin, formin, profilin, tropomyosin, capping protein, cofilin, and AIP1) are sufficient to reconstitute the formation of cables that undergo polarized turnover and maintain steady-state lengths similar to actin cables in vivo. Further, the removal of individual proteins from this simple in vitro reconstitution system leads to cable defects that closely approximate in vivo cable phenotypes caused by disrupting the corresponding genes. Thus, a limited set of molecular components is capable of self-organizing into dynamic, micron-scale actin structures with features similar to cables in living cells.

Published
2020

11. Myosin motor isoforms direct specification of actomyosin function by tropomyosins

Author

Matthew Lord, Luther W. Pollard, George G. Murray, and Joseph E. Clayton

Subjects
Gene isoform, Skeletal muscle, macromolecular substances, Cell Biology, Biology, musculoskeletal system, Tropomyosin, Cell biology, medicine.anatomical_structure, Structural Biology, Myosin, medicine, Cytoskeleton, Actin, Cytokinesis, Function (biology)
Abstract

Myosins and tropomyosins represent two cytoskeletal proteins that often work together with actin filaments in contractile and motile cellular processes. While the specialized role of tropomyosin in striated muscle myosin-II regulation is well characterized, its role in nonmuscle myosin regulation is poorly understood. We previously showed that fission yeast tropomyosin (Cdc8p) positively regulates myosin-II (Myo2p) and myosin-V (Myo52p) motors. To understand the broader implications of this regulation we examined the role of two mammalian tropomyosins (Tpm3.1cy/Tm5NM1 and Tpm4.2cy/Tm4) recently implicated in cancer cell proliferation and metastasis. Like Cdc8p, the Tpm3.1cy and Tpm4.2cy isoforms significantly enhance Myo2p and Myo52p motor activity, converting nonprocessive Myo52p molecules into processive motors that can walk along actin tracks as single molecules. In contrast to the positive regulation of Myo2p and Myo52p, Cdc8p and the mammalian tropomyosins potently inhibited skeletal muscle myosin-II, while having negligible effects on the highly processive mammalian myosin-Va. In support of a conserved role for certain tropomyosins in regulating nonmuscle actomyosin structures, Tpm3.1cy supported normal contractile ring function in fission yeast. Our work reveals that actomyosin regulation by tropomyosin is dependent on the myosin isoform, highlighting a general role for specific isoforms of tropomyosin in sorting myosin motor outputs.

Published
2015
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12. Fission yeast myosin Myo2 is down-regulated in actin affinity by light chain phosphorylation

Author

Susan Lowey, Elena B. Krementsova, Luther W. Pollard, Kathleen M. Trybus, Qing Tang, and Carol S. Bookwalter

Subjects
0301 basic medicine, Myosin Type V, Down-Regulation, Sf9, macromolecular substances, Biology, Myosins, 03 medical and health sciences, Contractile Proteins, Cell cortex, Myosin, Schizosaccharomyces, Amino Acid Sequence, Phosphorylation, Actin, Cytokinesis, Myosin Type II, Multidisciplinary, Myosin Heavy Chains, Microfilament Proteins, biology.organism_classification, Actins, Cell biology, Actin Cytoskeleton, Cytoskeletal Proteins, 030104 developmental biology, PNAS Plus, Chaperone (protein), Schizosaccharomyces pombe, biology.protein, Schizosaccharomyces pombe Proteins, Cell Division
Abstract

Studies in fission yeast Schizosaccharomyces pombe have provided the basis for the most advanced models of the dynamics of the cytokinetic contractile ring. Myo2, a class-II myosin, is the major source of tension in the contractile ring, but how Myo2 is anchored and regulated to produce force is poorly understood. To enable more detailed biochemical/biophysical studies, Myo2 was expressed in the baculovirus/Sf9 insect cell system with its two native light chains, Rlc1 and Cdc4. Milligram yields of soluble, unphosphorylated Myo2 were obtained that exhibited high actin-activated ATPase activity and in vitro actin filament motility. The fission yeast specific chaperone Rng3 was thus not required for expression or activity. In contrast to nonmuscle myosins from animal cells that require phosphorylation of the regulatory light chain for activation, phosphorylation of Rlc1 markedly reduced the affinity of Myo2 for actin. Another unusual feature of Myo2 was that, unlike class-II myosins, which generally form bipolar filamentous structures, Myo2 showed no inclination to self-assemble at approximately physiological salt concentrations, as analyzed by sedimentation velocity ultracentrifugation. This lack of assembly supports the hypothesis that clusters of Myo2 depend on interactions at the cell cortex in structural units called nodes for force production during cytokinesis.

Published
2017

14. Myosin motor isoforms direct specification of actomyosin function by tropomyosins

Author

Joseph E, Clayton, Luther W, Pollard, George G, Murray, and Matthew, Lord

Subjects
Adenosine Triphosphatases, Myosin Heavy Chains, Molecular Motor Proteins, Green Fluorescent Proteins, Myosin Type V, Cell Cycle Proteins, macromolecular substances, Actomyosin, Exons, Tropomyosin, Myosins, musculoskeletal system, Article, Actin Cytoskeleton, Cytoskeletal Proteins, Gene Expression Regulation, Cell Movement, Schizosaccharomyces, Escherichia coli, Humans, Protein Isoforms, Schizosaccharomyces pombe Proteins, Muscle, Skeletal, Plasmids
Abstract

Myosins and tropomyosins represent two cytoskeletal proteins that often work together with actin filaments in contractile and motile cellular processes. While the specialized role of tropomyosin in striated muscle myosin-II regulation is well characterized, its role in non-muscle myosin regulation is poorly understood. We previously showed that fission yeast tropomyosin (Cdc8p) positively regulates myosin-II (Myo2p) and myosin-V (Myo52p) motors. To understand the broader implications of this regulation we examined the role of two mammalian tropomyosins (Tpm3.1cy/Tm5NM1 and Tpm4.2cy/Tm4) recently implicated in cancer cell proliferation and metastasis. Like Cdc8p, the Tpm3.1cy and Tpm4.2cy isoforms significantly enhance Myo2p and Myo52p motor activity, converting non-processive Myo52p molecules into processive motors that can walk along actin tracks as single molecules. In contrast to the positive regulation of Myo2p and Myo52p, Cdc8p and the mammalian tropomyosins potently inhibited skeletal muscle myosin-II, while having negligible effects on the highly processive mammalian myosin-Va. In support of a conserved role for certain tropomyosins in regulating non-muscle actomyosin structures, Tpm3.1cy supported normal contractile ring function in fission yeast. Our work reveals that actomyosin regulation by tropomyosin is dependent on the myosin isoform, highlighting a general role for specific isoforms of tropomyosin in sorting myosin motor outputs.

Published
2014

15. Getting myosin-V on the right track: tropomyosin sorts transport in yeast

Author

Matthew Lord and Luther W. Pollard

Subjects
Cell Cycle Proteins, Cell Biology, General Medicine, Processivity, macromolecular substances, Articles, Biology, Myosins, musculoskeletal system, Tropomyosin, Yeast, Cell biology, Actin Cytoskeleton, Biochemistry, Structural Biology, Myosin, Schizosaccharomyces, Enzyme kinetics, Schizosaccharomyces pombe Proteins, Actin, Function (biology), Intracellular transport, Cytoskeleton
Abstract

Fission yeast tropomyosin targets myosin-V to actin cables by favoring processivity of the motor. Live-cell imaging is used to estimate the number of myosin-V molecules per motile particle in vivo. In vitro reconstitution demonstrates the physiological relevance of tropomyosin-based targeting of this motor., A hallmark of class-V myosins is their processivity—the ability to take multiple steps along actin filaments without dissociating. Our previous work suggested, however, that the fission yeast myosin-V (Myo52p) is a nonprocessive motor whose activity is enhanced by tropomyosin (Cdc8p). Here we investigate the molecular mechanism and physiological relevance of tropomyosin-mediated regulation of Myo52p transport, using a combination of in vitro and in vivo approaches. Single molecules of Myo52p, visualized by total internal reflection fluorescence microscopy, moved processively only when Cdc8p was present on actin filaments. Small ensembles of Myo52p bound to a quantum dot, mimicking the number of motors bound to physiological cargo, also required Cdc8p for continuous motion. Although a truncated form of Myo52p that lacked a cargo-binding domain failed to support function in vivo, it still underwent actin-dependent movement to polarized growth sites. This result suggests that truncated Myo52p lacking cargo, or single molecules of wild-type Myo52p with small cargoes, can undergo processive movement along actin-Cdc8p cables in vivo. Our findings outline a mechanism by which tropomyosin facilitates sorting of transport to specific actin tracks within the cell by switching on myosin processivity.

Published
2014

16. Fission yeast tropomyosin specifies directed transport of myosin-V along actin cables

Author

Matthew Lord, Alex R. Hodges, Kathleen M. Trybus, Luther W. Pollard, Joseph E. Clayton, Maria Sckolnick, and Carol S. Bookwalter

Subjects
Arp2/3 complex, Biological Transport, Active, Cell Cycle Proteins, macromolecular substances, Biology, Myosins, Time-Lapse Imaging, Adenosine Triphosphate, Myosin, Schizosaccharomyces, Protein Interaction Domains and Motifs, Actin-binding protein, Molecular Biology, Actin, Actin remodeling, Cell Biology, Processivity, Actin cytoskeleton, musculoskeletal system, Tropomyosin, Cell biology, Actin Cytoskeleton, Microscopy, Fluorescence, biology.protein, Commentary, Schizosaccharomyces pombe Proteins
Abstract

A hallmark of class-V myosins is their processivity—the ability to take multiple steps along actin filaments without dissociating. Our previous work suggested, however, that the fission yeast myosin-V (Myo52p) is a nonprocessive motor whose activity is enhanced by tropomyosin (Cdc8p). Here we investigate the molecular mechanism and physiological relevance of tropomyosin-mediated regulation of Myo52p transport, using a combination of in vitro and in vivo approaches. Single molecules of Myo52p, visualized by total internal reflection fluorescence microscopy, moved processively only when Cdc8p was present on actin filaments. Small ensembles of Myo52p bound to a quantum dot, mimicking the number of motors bound to physiological cargo, also required Cdc8p for continuous motion. Although a truncated form of Myo52p that lacked a cargo-binding domain failed to support function in vivo, it still underwent actin-dependent movement to polarized growth sites. This result suggests that truncated Myo52p lacking cargo, or single molecules of wild-type Myo52p with small cargoes, can undergo processive movement along actin-Cdc8p cables in vivo. Our findings outline a mechanism by which tropomyosin facilitates sorting of transport to specific actin tracks within the cell by switching on myosin processivity.

Published
2013

17. Myosin II Head Interaction in Primitive Species

Author

Kathleen M. Trybus, Kyounghwan Lee, Xiong Liu, Roger Craig, Floyd Sarsoza, Luther W. Pollard, Matthew Lord, Edward D. Korn, Sanford I. Bernstein, and Shixin Yang

Subjects
0301 basic medicine, Myosin light-chain kinase, Meromyosin, Biophysics, macromolecular substances, Biology, biology.organism_classification, Motor protein, Skeletal Muscle Myosins, 03 medical and health sciences, Myosin head, 030104 developmental biology, Biochemistry, Schizosaccharomyces pombe, Myosin, Actin
Abstract

Myosin II is a two-headed motor protein with an elongated α-helical tail. The motor domain of each head interacts with actin to convert the chemical energy of ATP into movement. Myosin II activity in muscle and nonmuscle cells is switched off by intramolecular interaction between its two heads, which inhibits their activity. This has been shown by EM and image processing of myosin filaments and isolated myosin molecules. In switched-off single molecules, the myosin tail folds into three segments, with the interacting heads folded back on the tail. The interacting-heads motif is highly conserved, being found in vertebrate and invertebrate smooth and striated muscle and in nonmuscle cells. We are investigating its evolutionary origins by EM imaging of isolated myosin molecules in the off-state. In previous work we found that the motif was present as far back as Cnidaria (sea anemones), the earliest animals with muscles. Here we have studied additional animal and non-animal species. At high (0.5 M) salt, all the myosin IIs showed the typical appearance of an extended tail and non-interacting heads. At low salt (0.15 M), under relaxing conditions (MgATP), insect indirect flight and embryonic skeletal muscle myosins showed a folded tail and similar head-head interactions to other muscles. Three species of primitive, non-animal myosins gave differing results. Acanthamoeba (reported previously) and Schizosaccharomyces pombe showed extended tails and no head-head interactions. The tails of these two myosins were approximately 30-40% shorter than the animal myosins, possibly accounting for their inability to fold. In contrast, Dictyostelium, with a tail 10% longer than animal myosin, showed head-head interactions similar to animal myosin; however, the conformation of the folded tail was different. These results suggest that head-head interaction arose before the evolution of animals.

Published
2016
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18. Fission yeast Cyk3p is a transglutaminase-like protein that participates in cytokinesis and cell morphogenesis

Author

Masayuki Onishi, Luther W. Pollard, John R. Pringle, and Matthew Lord

Subjects
Tissue transglutaminase, Recombinant Fusion Proteins, Green Fluorescent Proteins, Morphogenesis, Cell Cycle Proteins, Spindle Apparatus, Time-Lapse Imaging, 03 medical and health sciences, Gene Knockout Techniques, 0302 clinical medicine, Contractile Proteins, Cell polarity, Schizosaccharomyces, Cell Cycle Protein, Molecular Biology, 030304 developmental biology, Cytokinesis, Sequence Deletion, 0303 health sciences, biology, Cell morphogenesis, Cell Cycle, Cell Polarity, Cell Biology, Articles, biology.organism_classification, Cell biology, Transport protein, Protein Structure, Tertiary, Kinetics, Protein Transport, biology.protein, Schizosaccharomyces pombe Proteins, 030217 neurology & neurosurgery
Abstract

We have identified a fission yeast morphogenesis factor (Cyk3p) that functions with myosin II and chitin synthase during cytokinesis. Cyk3p possesses a novel transglutaminase domain that lacks an active site yet is essential for function. Our work demonstrates the physiological importance of such domains, which are found throughout eukaryotes., Cell morphogenesis is a complex process that relies on a diverse array of proteins and pathways. We have identified a transglutaminase-like protein (Cyk3p) that functions in fission yeast morphogenesis. The phenotype of a cyk3 knockout strain indicates a primary role for Cyk3p in cytokinesis. Correspondingly, Cyk3p localizes both to the actomyosin contractile ring and the division septum, promoting ring constriction, septation, and subsequent cell separation following ring disassembly. In addition, Cyk3p localizes to polarized growth sites and plays a role in cell shape determination, and it also appears to contribute to cell integrity during stationary phase, given its accumulation as dynamic puncta at the cortex of such cells. Our results and the conservation of Cyk3p across fungi point to a role in cell wall synthesis and remodeling. Cyk3p possesses a transglutaminase domain that is essential for function, even though it lacks the catalytic active site. In a wider sense, our work illustrates the physiological importance of inactive members of the transglutaminase family, which are found throughout eukaryotes. We suggest that the proposed evolution of animal transglutaminase cross-linking activity from ancestral bacterial thiol proteases was accompanied by the emergence of a subclass whose function does not depend on enzymatic activity.

Published
2012

19. Tropomyosin and myosin-II cellular levels promote actomyosin ring assembly in fission yeast

Author

Benjamin C. Stark, Thomas E. Sladewski, Matthew Lord, and Luther W. Pollard

Subjects
Recombinant Fusion Proteins, Motility, macromolecular substances, Tropomyosin, Protein filament, Myosin, Schizosaccharomyces, Molecular Biology, Actin, Cytoskeleton, Cytokinesis, Myosin Type II, biology, Myosin Heavy Chains, Fluorescence recovery after photobleaching, Cell Biology, Actomyosin, Articles, biology.organism_classification, musculoskeletal system, Cell biology, Schizosaccharomyces pombe Proteins, tissues, Fluorescence Recovery After Photobleaching
Abstract

A combination of in vivo and in vitro approaches were used to show how tropomyosin and myosin-II contribute to contractile ring assembly in fission yeast. Ring assembly is sensitive to changes in the cellular levels of myosin-II, and tropomyosin works to maximize myosin-II motor function during this process by stabilizing actomyosin interactions., Myosin-II (Myo2p) and tropomyosin are essential for contractile ring formation and cytokinesis in fission yeast. Here we used a combination of in vivo and in vitro approaches to understand how these proteins function at contractile rings. We find that ring assembly is delayed in Myo2p motor and tropomyosin mutants, but occurs prematurely in cells engineered to express two copies of myo2. Thus, the timing of ring assembly responds to changes in Myo2p cellular levels and motor activity, and the emergence of tropomyosin-bound actin filaments. Doubling Myo2p levels suppresses defects in ring assembly associated with a tropomyosin mutant, suggesting a role for tropomyosin in maximizing Myo2p function. Correspondingly, tropomyosin increases Myo2p actin affinity and ATPase activity and promotes Myo2p-driven actin filament gliding in motility assays. Tropomyosin achieves this by favoring the strong actin-bound state of Myo2p. This mode of regulation reflects a role for tropomyosin in specifying and stabilizing actomyosin interactions, which facilitates contractile ring assembly in the fission yeast system.

Published
2010

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