Protein Kinase C-θ Phosphorylation of Moesin in the Actin-binding Sequence

Pietromonaco, Salvatore F.; Simons, Peter C.; Altman, Amnon; Elias, Laurence

doi:10.1074/jbc.273.13.7594

Cited by 193 publications

(154 citation statements)

References 61 publications

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“…Phosphorylation represents one mechanism for regulating the function of ERM proteins by modulating the ability of these proteins to form FERM/C-term associations (Nakamura et al, 1995;Matsui et al, 1998;Oshiro et al, 1998;Pietromonaco et al, 1998;Tran Quang et al, 2000;Ng et al, 2001). When phosphorylated at threonine 558 (moesin), 567 (ezrin) or 564 (radixin), ERM proteins assume an open conformation and can interact with F-actin.…”

Section: Discussionmentioning

confidence: 99%

Effect of merlin phosphorylation on neurofibromatosis 2 (NF2) gene function

2004

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The neurofibromatosis 2 (NF2) tumor suppressor gene product, merlin, belongs to the ezrin-radixin-moesin (ERM) subgroup of the Protein 4.1 family, which links cell surface glycoproteins to the actin cytoskeleton. Previous studies have suggested that phosphorylation of merlin, similar to other ERM proteins, may regulate its function. To determine whether merlin phosphorylation has functional consequences for merlin suppression of cell growth and motility, we generated doxycycline-regulatable RT4 schwannoma cell lines that inducibly express full-length merlin with mutations at two potential phosphorylation sites (amino-acid residues S518 and T576). Whereas a mutation at S518 that mimics constitutive phosphorylation (S518D) abrogates the ability of merlin to suppress cell growth and motility, the S518A merlin mutant, which mimics nonphosphorylated merlin, functions equivalently to wild-type merlin. Similar mutations involving T576, the analogous phosphorylation site in ERM proteins important for regulating their function, had no effect. In contrast to other functionally inactive missense merlin mutants, the regulated overexpression of S518D merlin resulted in dramatic changes in cell shape and the elaboration of filopodial extensions. These results provide the first direct demonstration that the S518D merlin mutation, which mimics merlin phosphorylation, impairs not only merlin growth and motility suppression but also leads to an acquisition of a novel phenotype previously ascribed to ERM proteins.

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Section: Discussionmentioning

confidence: 99%

Effect of merlin phosphorylation on neurofibromatosis 2 (NF2) gene function

2004

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“…2 A and B). This preference is also shared by PKC-, another candidate ERM kinase (11,23,24). LOK too has a preference for basic residues, but the most prominent feature of LOK's peptide specificity is its strong and unusual preference for Y at P-2 (2 amino acids before the phosphorylation site), which is not shared by ROCK (Fig.…”

Section: Lok Has Strong Specificity For Erm Both At the Peptide And Pmentioning

confidence: 97%

LOK is a major ERM kinase in resting lymphocytes and regulates cytoskeletal rearrangement through ERM phosphorylation

Belkina

Liu

Hao

et al. 2009

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

123

129

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ERM (ezrin-radixin-moesin) proteins mediate linkage of actin cytoskeleton to plasma membrane in many cells. ERM activity is regulated in part by phosphorylation at a C-terminal threonine, but the identity of ERM kinases is unknown in lymphocytes and incompletely defined in other mammalian cells. Our studies show that lymphocyte-oriented kinase (LOK) is an ERM kinase in vitro and in vivo. Mass spectrometric analysis indicates LOK is abundant at the lymphocyte plasma membrane and immunofluorescence studies show LOK enrichment at the plasma membrane near ERM. In vitro peptide specificity analyses characterize LOK as a basophilic kinase whose optimal substrate sequence resembles the ERM site, including unusual preference for tyrosine at P-2. LOK's activity on moesin peptide and protein was comparable to reported ERM kinases ROCK and PKC but unlike them LOK displayed preferential specificity for moesin compared to traditional basophilic kinase substrates. Two genetic approaches demonstrate a role for LOK in ERM phosphorylation: cell transfection with LOK kinase domain augments ERM phosphorylation and lymphocytes from LOK knockout mice have >50% reduction in ERM phosphorylation. The findings on localization and specificity argue that LOK is a direct ERM kinase. The knockout mice have normal hematopoietic cell development but notably lymphocyte migration and polarization in response to chemokine are enhanced. These functional alterations fit the current understanding of the role of ERM phosphorylation in regulating cortical reorganization. Thus, these studies identify a new ERM kinase of importance in lymphocytes and confirm the role of ERM phosphorylation in regulating cell shape and motility.ezrin ͉ kinase specificity ͉ knockout ͉ migration ͉ moesin T he ERM family in mammals consists of 3 closely related members: ezrin, radixin and moesin whose major function is to link cortical actin filaments to the plasma membrane (1-4). ERM N terminus (the FERM/band 4.1 domain) binds to plasma membrane both by direct interaction with phospholipids and by binding cytoplasmic tails of transmembrane proteins such as CD43, CD44, and ICAMs. ERM C terminus (''tail'') binds to filamentous actin. ERMs exist not only in this active conformation, but also in an inactive conformation where the C terminus binds to the FERM domain, thereby blocking binding sites on both FERM and tail. There is an evolutionarily conserved phosphorylation site near the C terminus whose phosphorylation contributes to stabilizing the active conformation. In mitotic cells ERM phosphorylation is critical for achieving spherical morphology and rigidity (5, 6). For lymphocytes circulating in blood, ERM phosphorylation is understood to contribute to rigidity and maintenance of microvilli. In response to chemotactic factors (especially chemokines) those lymphocytes transition into flexible migrating cells concurrent with rapid extensive dephosphorylation of ERM, which facilitates their polarization (7-10).Given the importance of ERM phosphorylation, it is essential to...

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“…Activation of ERM proteins occurs by conformational changes triggered by binding of phosphatidylinositol 4,5-biphosphate (PIP 2 ) to the FERM (band 4.1, ERM) domain in the NH 2 -terminal region, termed the NH 2 -terminal ERM-associated domain (N-ERMAD) and phosphorylation of a conserved threonine residue (ezrin-T567, radixin-T564, moesin-T558) in the COOH-terminal domain, termed the COOH-terminal ERMassociated domain (C-ERMAD; Pietromonaco et al, 1998;Barret et al, 2000;Ng et al, 2001;Fievet et al, 2004). This sequence of molecular events releases the intramolecular interaction between the N-and C-termini.…”

Section: Introductionmentioning

confidence: 99%

Activated Ezrin Promotes Cell Migration through Recruitment of the GEF Dbl to Lipid Rafts and Preferential Downstream Activation of Cdc42

Prag

Parsons

Keppler

et al. 2007

MBoC

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Establishment of polarized cell morphology is a critical factor for migration and requires precise spatial and temporal activation of the Rho GTPases. Here, we describe a novel role of the actin-binding ezrin/radixin/moesin (ERM)-protein ezrin to be involved in recruiting Cdc42, but not Rac1, to lipid raft microdomains, as well as the subsequent activation of this Rho GTPase and the downstream effector p21-activated kinase (PAK)1, as shown by fluorescence lifetime imaging microscopy. The establishment of a leading plasma membrane and the polarized morphology necessary for random migration are also dependent on ERM function and Cdc42 in motile breast carcinoma cells. Mechanistically, we show that the recruitment of the ERM-interacting Rho/Cdc42-specific guanine nucleotide exchange factor Dbl to the plasma membrane and to lipid raft microdomains requires the phosphorylated, active conformer of ezrin, which serves to tether the plasma membrane or its subdomains to the cytoskeleton. Together these data suggest a mechanism whereby precise spatial guanine nucleotide exchange of Cdc42 by Dbl is dependent on functional ERM proteins and is important for directional cell migration.

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Protein Kinase C-θ Phosphorylation of Moesin in the Actin-binding Sequence

Cited by 193 publications

References 61 publications

Effect of merlin phosphorylation on neurofibromatosis 2 (NF2) gene function

Effect of merlin phosphorylation on neurofibromatosis 2 (NF2) gene function

LOK is a major ERM kinase in resting lymphocytes and regulates cytoskeletal rearrangement through ERM phosphorylation

Activated Ezrin Promotes Cell Migration through Recruitment of the GEF Dbl to Lipid Rafts and Preferential Downstream Activation of Cdc42

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