A novel member of the rho family of small GTP-binding proteins is specifically required for cytokinesis.

Larochelle, Denis A.; Vithalani, Kalpa K.; Lozanne, Arturo De

doi:10.1083/jcb.133.6.1321

Cited by 131 publications

(125 citation statements)

References 39 publications

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“…(2) Mutants altered in proteins that play a regulatory role in mitosis. Coronin, a WD40-repeat protein involved in dynamic rearrangements of the actin system [23], racE [24], and DGAP1 belong to this category. These and certainly more regulatory proteins are required in D. discoideum cells to guarantee the coordination in time and space of cytoskeletal activities in the cell cortex.…”

Section: Discussionmentioning

confidence: 99%

DGAP1, a homologue of rasGTPase activating proteins that controls growth, cytokinesis, and development in Dictyostelium discoideum

Faix

Dittrich

1996

FEBS Letters

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Section: Discussionmentioning

confidence: 99%

DGAP1, a homologue of rasGTPase activating proteins that controls growth, cytokinesis, and development in Dictyostelium discoideum

Faix

Dittrich

1996

FEBS Letters

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“…The distribution of GFP-N25racE in these cells remained unchanged, localizing primarily to the plasma membrane in both interphase and dividing cells ( Figure 5, B, C, E, and F). Localization of GFP-racE Is Mediated by the C Terminus of racE Although all members of the rho family of small GTPases are very similar to each other, a salient feature of racE is the unique sequence near its carboxyl terminus (Larochelle et al, 1996). In comparison to all other members of this family, the C-terminal domain of racE is extended by about 28 amino acids.…”

Section: Growth Curvesmentioning

confidence: 99%

“…The active mutant is the result of reduced GTPase activity (Garrett et al, 1989) and the inactive mutant is the result of an inability to exchange GTP for bound GDP (Feig and Cooper, 1988). A fusion protein was also designed, using PCR, to replace the short hypervariable carboxyl-terminal region of racC with the extended carboxyl-terminal region of racE (Larochelle et al, 1996). This protein, named racC/E tail, contained amino acid residues 1-180 of racC and residues 184-223 of racE.…”

Section: Materials and Methods Mutant And Gfp Expression Constructsmentioning

confidence: 99%

“…The Function of racE Cannot Be Replaced by a Closely Related Protein Currently, the protein most similar to Dictyostelium racE in the GenBank database is the Dictyostelium racC protein (Bush et al, 1993;Larochelle et al, 1996). Although racC shares 54% identical residues (68% overall conserved) with racE, it apparently cannot substi- tute for racE in cytokinesis since racC is expressed in racE null cells.…”

Section: Growth Curvesmentioning

confidence: 99%

“…Recently, using a genetic screen for Dictyostelium cytokinesis mutants, we identified a novel member of the rho family of GTPases, which we designated as racE (Larochelle et al, 1996). This protein appears to have a specific role during cytokinesis since a null mutation in the racE gene does not perturb any cellular event except for cell division.…”

Section: Introductionmentioning

confidence: 99%

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Role of Dictyostelium racE in cytokinesis: mutational analysis and localization studies by use of green fluorescent protein.

Larochelle

Vithalani

Lozanne

1997

MBoC

Self Cite

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The small GTPase racE is essential for cytokinesis in Dictyostelium but its precise role in cell division is not known. To determine the molecular mechanism of racE function, we undertook a mutational analysis of racE. The exogenous expression of either wild-type racE or a constitutively active V20racE mutant effectively rescues the cytokinesis deficiency of racE null cells. In contrast, a constitutively inactive N25racE mutant fails to rescue the cytokinesis deficiency. Thus, cytokinesis requires only the activation of racE by GTP and not the inactivation of racE by hydrolysis of GTP. To determine the spatial distribution of racE, we created a fusion protein with GFP at the amino terminus of racE. Remarkably, GFP-racE fusion protein was fully competent to rescue the phenotype of racE null cells and, therefore, must reside in the same location as native racE. We found that GFP-racE localized to the plasma membrane of the cell throughout the entire cell cycle. Furthermore, constitutively active and inactive GFP-racE fusion proteins also localized to the plasma membrane. We mapped the domain required for plasma membrane localization to the carboxyl-terminal 40 amino acids of racE. This domain, however, is not sufficient to confer racE function onto a closely related GTPase. Taken together, these results suggest that racE functions at the cell cortex but it is not involved in determining the timing or placement of the contractile ring.

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Molecular biological approaches to study myosin functions in cytokinesis ofDictyostelium

Uyeda¹,

Yumura

2000

Microsc. Res. Tech.

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A novel member of the rho family of small GTP-binding proteins is specifically required for cytokinesis.

Cited by 131 publications

References 39 publications

DGAP1, a homologue of rasGTPase activating proteins that controls growth, cytokinesis, and development in Dictyostelium discoideum

DGAP1, a homologue of rasGTPase activating proteins that controls growth, cytokinesis, and development in Dictyostelium discoideum

Role of Dictyostelium racE in cytokinesis: mutational analysis and localization studies by use of green fluorescent protein.

Molecular biological approaches to study myosin functions in cytokinesis ofDictyostelium

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