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Uncovering a Role for the Tail of the Dictyostelium discoideum SadA Protein in Cell-Substrate Adhesion

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ABSTRACTPrevious work from our laboratory showed that theDictyostelium discoideumSadA protein plays a central role in cell-substrate adhesion. SadA null cells exhibit a loss of adhesion, a disrupted actin cytoskeleton, and a cytokinesis defect. How SadA mediates these phenotypes is unknown. This work addresses the mechanism of SadA function, demonstrating an important role for the C-terminal cytoplasmic tail in SadA function. We found that a SadA tailless mutant was unable to rescue thesadAadhesion deficiency, and overexpression of the SadA tail domain reduced adhesion in wild-type cells. We also show that SadA is closely associated with the actin cytoskeleton. Mutagenesis studies suggested that four serine residues in the tail, S924/S925 and S940/S941, may regulate association of SadA with the actin cytoskeleton. GlutathioneS-transferase pull-down assays identified at least one likely interaction partner of the SadA tail, cortexillin I, a known actin bundling protein. Thus, our data demonstrate an important role for the carboxy-terminal cytoplasmic tail in SadA function and strongly suggest that a phosphorylation event in this tail regulates an interaction with cortexillin I. Based on our data, we propose a model for the function of SadA.
American Society for Microbiology
Title: Uncovering a Role for the Tail of the Dictyostelium discoideum SadA Protein in Cell-Substrate Adhesion
Description:
ABSTRACTPrevious work from our laboratory showed that theDictyostelium discoideumSadA protein plays a central role in cell-substrate adhesion.
SadA null cells exhibit a loss of adhesion, a disrupted actin cytoskeleton, and a cytokinesis defect.
How SadA mediates these phenotypes is unknown.
This work addresses the mechanism of SadA function, demonstrating an important role for the C-terminal cytoplasmic tail in SadA function.
We found that a SadA tailless mutant was unable to rescue thesadAadhesion deficiency, and overexpression of the SadA tail domain reduced adhesion in wild-type cells.
We also show that SadA is closely associated with the actin cytoskeleton.
Mutagenesis studies suggested that four serine residues in the tail, S924/S925 and S940/S941, may regulate association of SadA with the actin cytoskeleton.
GlutathioneS-transferase pull-down assays identified at least one likely interaction partner of the SadA tail, cortexillin I, a known actin bundling protein.
Thus, our data demonstrate an important role for the carboxy-terminal cytoplasmic tail in SadA function and strongly suggest that a phosphorylation event in this tail regulates an interaction with cortexillin I.
Based on our data, we propose a model for the function of SadA.

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