Functions of the novel RhoGAP proteins RGA-3 and RGA-4 in the germ line and in the early embryo of<i>C. elegans</i>

Schmutz, Cornelia; Stevens, Julia; Spang, Anne

doi:10.1242/dev.000802

Cited by 60 publications

(68 citation statements)

References 38 publications

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“…1D). Similar PAR domain size correction can be observed in other mutants with enlarged posterior domains, such as rga-3/4(RNAi) embryos (Schmutz et al, 2007;Schonegg et al, 2007), in two-cell embryos with spindle orientation defects (Gomes et al, 2001) and in subsequent divisions of the germline lineage in wild-type C. elegans embryos (see Figs S1 and S2 in the supplementary material; see Movie 2 in the supplementary material). C. elegans embryos appear to match the PAR domain boundary to the site of cell division.…”

Section: The Site Of Cell Division Repositions the Par Domain Boundarysupporting

confidence: 71%

Cortical domain correction repositions the polarity boundary to match the cytokinesis furrow in C. elegans embryos

et al. 2010

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SUMMARYIn asymmetrically dividing cells, a failure to coordinate cell polarity with the site of cell division can lead to cell fate transformations and tumorigenesis. Cell polarity in C. elegans embryos is defined by PAR proteins, which occupy reciprocal halves of the cell cortex. During asymmetric division, the boundary between the anterior and posterior PAR domains precisely matches the site of cell division, ensuring exclusive segregation of cell fate. The PAR domains determine the site of cell division by positioning the mitotic spindle, suggesting one means by which cell polarity and cell division might be coordinated. Here, we report that cell polarity and cell division are coordinated through an additional mechanism: the site of cell division repositions the PAR-2 boundary. G-mediated microtubule-cortex interactions appear to direct cortical flows of PAR-2 and myosin toward the site of cell division, which acts as a PAR-2 and myosin sink. Embryos with defects in PAR-2 boundary correction undergo mis-segregation of cortical polarity and cytoplasmic determinants, suggesting that PAR domain correction might help prevent cell fate transformation.

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Section: The Site Of Cell Division Repositions the Par Domain Boundarysupporting

confidence: 71%

Cortical domain correction repositions the polarity boundary to match the cytokinesis furrow in C. elegans embryos

et al. 2010

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“…These challenges have made it difficult to determine whether CYK-4 corresponds to the centrosome-dependent polarization cue, or if CYK-4 and the centrosome cue function in parallel. The functionally redundant RhoGAP proteins RGA-3 and RGA-4 (hereafter RGA-3/4) attenuate myosin activity to limit the extent of actomyosin contraction (Schmutz et al, 2007;Schonegg et al, 2007). In rga-3/4(RNAi) embryos, the myosin network is more dense and filamentous and contracts too far anteriorly, creating a smaller anterior PAR domain.…”

Section: Actomyosin Regulation During the Establishment Phasementioning

confidence: 99%

Elaborating polarity: PAR proteins and the cytoskeleton

Nance¹,

2011

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Cell polarity is essential for cells to divide asymmetrically, form spatially restricted subcellular structures and participate in three-dimensional multicellular organization. PAR proteins are conserved polarity regulators that function by generating cortical landmarks that establish dynamic asymmetries in the distribution of effector proteins. Here, we review recent findings on the role of PAR proteins in cell polarity in C. elegans and Drosophila, and emphasize the links that exist between PAR networks and cytoskeletal proteins that both regulate PAR protein localization and act as downstream effectors to elaborate polarity within the cell.

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“…However, CYK-4 is also a component of a complex involved in cytokinesis, and in this situation, at least, it is specific for Rac inactivation rather than Rho-1 (Canman et al 2008). Two other RhoGAPs are present in C. elegans but seem to have a distinct function from CYK-4 because they control the ratio of the anterior/posterior domain rather than its formation (Schmutz et al 2007;Schonegg et al 2007). Rho-1 GTP normally activates a downstream kinase that phosphorylates myosin light chain, increasing contractility, but the accumulation of the GAP depletes Rho-GTP and relaxes actomyosin at the posterior cortex.…”

Section: Polarity Signaling Through Par-3/par-6/apkcmentioning

confidence: 99%