4.5 Article

Costars, a Dictyostelium protein similar to the C-terminal domain of STARS, regulates the actin cytoskeleton and motility

期刊

JOURNAL OF CELL SCIENCE
卷 123, 期 21, 页码 3745-3755

出版社

COMPANY OF BIOLOGISTS LTD
DOI: 10.1242/jcs.064709

关键词

Cell migration; Chemotaxis; Cytoskeleton; Pseudopod; Signal transduction

资金

  1. National Health Research Institutes, Taiwan [NHRI-EX92-9230SI, NHRI-EX93-9230SI, NHRI-EX94-9230SI]
  2. National Science Council [NSC97-2320-B-010-021, NSC 98-2320-B-010-023-MY3]
  3. Ministry of Education, Taiwan

向作者/读者索取更多资源

Through analysis of a chemotaxis mutant obtained from a genetic screen in Dictyostelium discoideum, we have identified a new gene involved in regulating cell migration and have named it costars (cosA). The 82 amino acid Costars protein sequence appears highly conserved among diverse species, and significantly resembles the C-terminal region of the striated muscle activator of Rho signaling (STARS), a mammalian protein that regulates the serum response factor transcriptional activity through actin binding and Rho GTPase activation. The cosA-null (cosA(-)) cells formed smooth plaques on bacterial lawns, produced abnormally small fruiting bodies when developed on the non-nutrient agar and displayed reduced migration towards the cAMP source in chemotactic assays. Analysis of cell motion in cAMP gradients revealed decreased speed but wild-type-like directional persistence of cosA-cells, suggesting a defect in the cellular machinery for motility rather than for chemotactic orientation. Consistent with this notion, cosA-cells exhibited changes in the actin cytoskeleton, showing aberrant distribution of F-actin in fluorescence cell staining and an increased amount of cytoskeleton-associated actin. Excessive pseudopod formation was also noted in cosA(-) cells facing chemoattractant gradients. Expressing cosA or its human counterpart mCostars eliminated abnormalities of cosA(-) cells. Together, our results highlight a role for Costars in modulating actin dynamics and cell motility.

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