Tropomodulin 3 Binds to Actin Monomers

Fischer, R.; Yarmola, Elena G.; Weber, K; Speicher, Kaye D.; Speicher, David W.; Bubb, Michael R.; Fowler, Velia M.

doi:10.1074/jbc.m606315200

Cited by 50 publications

(91 citation statements)

References 48 publications

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“…The MciZ-mediated increase of the apparent critical concentration of FtsZ for GTP hydrolysis suggests that a sequestration mechanism may operate at high concentrations of this antagonist (49). The combination of capping and sequestration effects has been also described for other cytoskeletal modulatory proteins (52). It remains to be determined whether a capping-like mechanism might explain the inhibition of FtsZ polymerization by substoichiometric levels of antagonists such as Kil.…”

Section: Discussionmentioning

confidence: 95%

Evidence That Bacteriophage λ Kil Peptide Inhibits Bacterial Cell Division by Disrupting FtsZ Protofilaments and Sequestering Protein Subunits

Hernández-Rocamora

Alfonso

Margolin

et al. 2015

Journal of Biological Chemistry

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Background: Kil peptide from bacteriophage targets FtsZ to prevent host cell division. Results: Kil disrupts FtsZ protofilaments producing shorter oligomers of variable size with reduced GTPase activity. Conclusion: At high concentrations, Kil likely inhibits FtsZ assembly via a subunit sequestration mechanism. Significance: This is the first biophysical study of how a bacteriophage disruptor of bacterial division inhibits FtsZ assembly.

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Section: Discussionmentioning

confidence: 95%

Evidence That Bacteriophage λ Kil Peptide Inhibits Bacterial Cell Division by Disrupting FtsZ Protofilaments and Sequestering Protein Subunits

Hernández-Rocamora

Alfonso

Margolin

et al. 2015

Journal of Biological Chemistry

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“…Cytoskeletal modulatory proteins rarely have a single effect on their targets and it is not unexpected that a capper may also exhibit sequestration effects. For example, tropomodulin, which is a minus-end capper like MciZ, has been shown to bind to actin monomers and promote sequestration at high concentrations (53). MciZ behaves as a sequesterer at high concentrations, as demonstrated by the increase in Cc app that is approximately equal to the concentration of added MciZ (Fig.…”

Section: Discussionmentioning

confidence: 99%

FtsZ filament capping by MciZ, a developmental regulator of bacterial division

Bisson‐Filho

Discola

Castellen

et al. 2015

Proc. Natl. Acad. Sci. U.S.A.

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Cytoskeletal structures are dynamically remodeled with the aid of regulatory proteins. FtsZ (filamentation temperature-sensitive Z) is the bacterial homolog of tubulin that polymerizes into rings localized to cell-division sites, and the constriction of these rings drives cytokinesis. Here we investigate the mechanism by which the Bacillus subtilis cell-division inhibitor, MciZ (mother cell inhibitor of FtsZ), blocks assembly of FtsZ. The X-ray crystal structure reveals that MciZ binds to the C-terminal polymerization interface of FtsZ, the equivalent of the minus end of tubulin. Using in vivo and in vitro assays and microscopy, we show that MciZ, at substoichiometric levels to FtsZ, causes shortening of protofilaments and blocks the assembly of higher-order FtsZ structures. The findings demonstrate an unanticipated capping-based regulatory mechanism for FtsZ.T he discovery that bacteria have actin-, tubulin-, and intermediate filament-like proteins demonstrated that the cytoskeleton is an ancient invention, predating the divergence between prokaryotes and eukaryotes (1). The GTPase FtsZ (filamentation temperature-sensitive Z) was the first prokaryotic protein to be recognized as a cytoskeletal element (2, 3). FtsZ is a tubulin-like protein, which is widely conserved in bacteria and the main component of the bacterial cytokinesis machine, or "divisome." FtsZ self-assembles into single-stranded protofilaments and these associate further inside cells to form a superstructure known as the Z ring (4, 5). FtsZ alone can generate a constriction force to initiate division (6). The Z ring also provides a scaffold onto which several other components of the divisome-mostly cell wall synthesizing enzymes-are recruited and oriented so as to build the division septum, a cross-wall separating a progenitor cell into two isogenic daughter cells (7).FtsZ and tubulin share several essential properties: their assembly is cooperative, stimulated by GTP, and leads to GTP hydrolysis; they form dynamic polymers whose turnover is dependent on nucleotide hydrolysis (8); they use essentially the same bond for polymer formation (9); and recent evidence indicates that they undergo similar allosteric transitions upon polymerization (10, 11). Not surprisingly, however, the functional specialization of these proteins led to some significant differences between them, the most prominent being that FtsZ exists as single protofilaments, whereas tubulin always adopts a multifilament tubular structure. This difference in their higherorder structure implies that the reactions that lead to cooperativity and subunit turnover are likely different. It has also represented a significant technical challenge for the study of FtsZ. Because FtsZ filaments are smaller than the resolution of optical microscopy, so far it has been impossible to determine essential properties associated with its dynamic behavior.Similarly to actin filaments and microtubules, the assembly of FtsZ protofilaments into a Z ring is regulated by a number of proteins that bind directly...

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“…Because Tmod3 mRNA is expressed ubiquitously in most cells and tissues, 12,47 we speculate that Tmod3 protein may be produced in erythroblast progenitors but only be recruited into the membrane skeleton to cap actin filament pointed ends when Tmod1 is lacking. Insufficient levels or altered properties of Tmod3 48,49 as the membrane skeleton assembles during late stages of erythroblast terminal maturation may lead to aberrant actin filament assembly, resulting in abnormal spectrin-actin lattice organization in mature RBCs. Alternatively, actin filaments may assemble normally into the membrane skeleton during differentiation in the absence of Tmod1 but undergo length redistribution during shear stress in the circulation because of insufficient capping by low levels of Tmod3.…”

Section: Discussionmentioning

confidence: 99%

Tropomodulin 1-null mice have a mild spherocytic elliptocytosis with appearance of Tropomodulin 3 in red blood cells and disruption of the membrane skeleton

Moyer

Nowak

Kim

et al. 2010

Blood

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150

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The short actin filaments in the red blood cell (RBC) membrane skeleton are capped at their pointed ends by tropomodulin 1 (Tmod1) and coated with tropomyosin (TM) along their length. Tmod1-TM control of actin filament length is hypothesized to regulate spectrin-actin lattice organization and membrane stability. We used a Tmod1 knockout mouse to investigate the in vivo role of Tmod1 in the RBC membrane skeleton. Western blots of Tmod1-null RBCs confirm the absence of Tmod1 and show the presence of Tmod3, which is normally not present in RBCs. Tmod3 is present at only one-fifth levels of Tmod1 present on wild-type membranes, but levels of actin, TMs, adducins, and other membrane skeleton proteins remain unchanged. Electron microscopy shows that actin filament lengths are more variable with spectrin-actin lattices displaying abnormally large and more variable pore sizes. Tmod1-null mice display a mild anemia with features resembling hereditary spherocytic elliptocytosis, including decreased RBC mean corpuscular volume, cellular dehydration, increased osmotic fragility, reduced deformability, and heterogeneity in osmotic ektacytometry. Insufficient capping of actin filaments by Tmod3 may allow greater actin dynamics at pointed ends, resulting in filament length redistribution, leading to irregular and attenuated spectrin-actin lattice connectivity, and concomitant RBC membrane instability.(Blood. 2010;116(14): 2590-2599) IntroductionThe membrane skeleton is composed of a highly cross-linked network of spectrin, actin filaments, and accessory proteins that underlies the plasma membrane of differentiated cells. This network creates membrane domains by anchoring and restricting the long-range distribution of membrane proteins and plays an important role in determining cell shapes, membrane contours, and mechanical properties. 1,2 The organization of the membrane skeleton is best known in red blood cells (RBCs), where it is organized as a quasi-hexagonal network with connecting strands formed by long, flexible spectrin molecules and vertices formed by short actin filaments. 3-5 Each short actin filament forms the core of a junctional complex with 2 rod-shaped tropomyosin (TM) molecules along the filament, 2 tropomodulin 1 (Tmod1) molecules capping the pointed filament end and an ␣/␤-adducin heterodimer capping the barbed filament end. 6,7 Dematin (protein 4.9) is also associated with the short actin filaments as are ␤1-spectrin protein 4.1R complexes that extend from the sides of the filaments to form the extended spectrin-actin network. The network is connected to membrane macromolecular complexes by multiple linkages: from ␤-spectrin by ankryin to band 3, and from the junctional complex by protein 4.1, ␣/␤-adducin and dematin to band 3, glycophorin C, the glucose transporter, and other components. 8 Disruptions either of attachments of the spectrin-actin lattice to membrane macromolecular complexes ("vertical" connections), or linkages within the plane of the spectrin-actin lattice ("horizontal" connections) lead to ...

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Tropomodulin 3 Binds to Actin Monomers

Cited by 50 publications

References 48 publications

Evidence That Bacteriophage λ Kil Peptide Inhibits Bacterial Cell Division by Disrupting FtsZ Protofilaments and Sequestering Protein Subunits

Evidence That Bacteriophage λ Kil Peptide Inhibits Bacterial Cell Division by Disrupting FtsZ Protofilaments and Sequestering Protein Subunits

FtsZ filament capping by MciZ, a developmental regulator of bacterial division

Tropomodulin 1-null mice have a mild spherocytic elliptocytosis with appearance of Tropomodulin 3 in red blood cells and disruption of the membrane skeleton

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