Plakoglobin interacts with and increases the protein levels of metastasis suppressor Nm23-H2 and regulates the expression of Nm23-H1

Aktary, Zackie; Chapman, Kimberly A.; Lam, Le Thanh; Lo, Andy; Ji, Ce; Graham, Kathryn; Cook, Leah M.; Li, L; Mackey, John R.; Pasdar, Manijeh

doi:10.1038/onc.2009.495

Cited by 52 publications

(59 citation statements)

References 68 publications

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“…ATP is required for phosphorylation of MLC by MLCK, and we therefore explored the possible role of Nm23, a member of the nucleoside diphosphate kinase (NDPK) family, which was recently identified as a partner of c-catenin in tumor cells (Aktary et al, 2010). Nm23 could be found at endothelial junctions together with EMMPRIN and c-catenin, and knockdown of either of these proteins resulted in a significant decrease in Nm23 localization to these sites.…”

Section: Discussionmentioning

confidence: 99%

“…An EMMPRIN-c-catenin-Nm23 complex regulates actomyosin contractility at endothelial cell junctions through local ATP production Given that actomyosin contractility requires ATP, we next investigated the possible role at the junction of the reported ccatenin partner nucleoside diphosphate kinase Nm23 (Aktary et al, 2010), which is able to generate ATP by exchanging phosphate groups from NTP to ADP. The presence of Nm23 in the EMMPRIN molecular complex was confirmed by coimmunoprecipitation from endothelial cell lysates (Fig.…”

Section: Emmprin Associates With C-catenin At Endothelial Junctionsmentioning

confidence: 99%

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An EMMPRIN/γ-catenin/Nm23 complex drives ATP production and actomyosin contractility at endothelial junctions

Moreno

Gonzalo

Gómez-Escudero

et al. 2014

Journal of Cell Science

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Cell-cell adhesions are important sites through which cells experience and resist forces. In endothelial cells, these forces regulate junction dynamics and determine endothelial barrier strength. We identify the Ig superfamily member EMMPRIN (also known as basigin) as a coordinator of forces at endothelial junctions. EMMPRIN localization at junctions correlates with endothelial junction strength in different mouse vascular beds. Accordingly, EMMPRIN-deficient mice show altered junctions and increased junction permeability. Lack of EMMPRIN alters the localization and function of VE-cadherin (also known as cadherin-5) by decreasing both actomyosin contractility and tugging forces at endothelial cell junctions. EMMPRIN ensures proper actomyosin-driven maturation of competent endothelial junctions by forming a molecular complex with c-catenin (also known as junction plakoglobin) and Nm23 (also known as NME1), a nucleoside diphosphate kinase, thereby locally providing ATP to fuel the actomyosin machinery. These results provide a novel mechanism for the regulation of actomyosin contractility at endothelial junctions and might have broader implications in biological contexts such as angiogenesis, collective migration and tissue morphogenesis by coupling compartmentalized energy production to junction assembly.

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Section: Discussionmentioning

confidence: 99%

Section: Emmprin Associates With C-catenin At Endothelial Junctionsmentioning

confidence: 99%

An EMMPRIN/γ-catenin/Nm23 complex drives ATP production and actomyosin contractility at endothelial junctions

Moreno

Gonzalo

Gómez-Escudero

et al. 2014

Journal of Cell Science

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Section: Abstract: Armadillo Protein Desmosome Extracellular Matrimentioning

confidence: 99%

“…PG is also found in the cytoplasm and nucleus (Green and Simpson, 2007;Schmidt and Koch, 2007), where it is able to act independently of its function in intercellular adhesion. Its adhesionindependent functions are still not well defined, but the data suggest that PG can regulate gene expression and protein stability (Aktary et al, 2010;Hakimelahi et al, 2000;Shimizu et al, 2008) in both a -catenin-dependent and -independent manner (Raurell et al, 2006;Teuliere et al, 2004;Yin and Green, 2004;Zhurinsky et al, 2000).Recently we demonstrated that PG not only inhibits motility of keratinocytes in contact, but also inhibits Src-dependent single cell motility (Yin et al, 2005b). The observed changes in motility and altered cell morphology of PG -/-keratinocytes suggested to us that PG could be regulating cell-substrate interactions by modulating components of the extracellular matrix (ECM), its integrin receptors and/or the molecules involved in ECM-triggered motility cues.…”

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confidence: 99%

Plakoglobin regulates cell motility through Rho- and fibronectin-dependent Src signaling

Todorović

Desai

Patterson

et al. 2010

Journal of Cell Science

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SummaryWe previously showed that the cell-cell junction protein plakoglobin (PG) not only suppresses motility of keratinocytes in contact with each other, but also, unexpectedly, of single cells. Here keratinocytes. PG -/-cells also exhibited Src-independent activation of the small GTPases Rac1 and RhoA. Both Src and RhoA inhibition attenuated PG -/-keratinocyte motility. We propose a novel role for PG in regulating cell motility through distinct ECM-Src and RhoGTPase-dependent pathways, influenced in part by PG-dependent regulation of FN mRNA stability. Key words: Armadillo protein, Desmosome, Extracellular matrix, KeratinocyteJournal of Cell Science (Caldelari et al., 2001) and adhesive strength (Acehan et al., 2008) in keratinocytes lacking PG. Moreover, PG-null mice and patients with pathogenic homozygous PG mutations have impaired tissue integrity associated with skin and heart defects (Aberle et al., 1995;Bierkamp et al., 1996;McKoy et al., 2000;Ruiz et al., 1996). PG is also found in the cytoplasm and nucleus (Green and Simpson, 2007;Schmidt and Koch, 2007), where it is able to act independently of its function in intercellular adhesion. Its adhesionindependent functions are still not well defined, but the data suggest that PG can regulate gene expression and protein stability (Aktary et al., 2010;Hakimelahi et al., 2000;Shimizu et al., 2008) in both a -catenin-dependent and -independent manner (Raurell et al., 2006;Teuliere et al., 2004;Yin and Green, 2004;Zhurinsky et al., 2000).Recently we demonstrated that PG not only inhibits motility of keratinocytes in contact, but also inhibits Src-dependent single cell motility (Yin et al., 2005b). The observed changes in motility and altered cell morphology of PG -/-keratinocytes suggested to us that PG could be regulating cell-substrate interactions by modulating components of the extracellular matrix (ECM), its integrin receptors and/or the molecules involved in ECM-triggered motility cues. Using a combination of live cell imaging and cross plating, we show here that PG expression has a potent impact on the organization of actin, its associated membrane protrusions, focal adhesions and Src-dependent motility, in large part through regulation of the expression levels of the underlying ECM components. In particular, the ability of PG to regulate fibronectin (FN; also know as Fn1) mRNA stability was identified as a novel mechanism contributing to PG-dependent suppression of keratinocyte motility. Further analysis indicated that PG-dependent alterations in activity of the small GTPases Rac1 and RhoA act in parallel with FN/Src-dependent regulation of cortical actin 3577 Plakoglobin regulates motility via ECM structures to fine tune the motile behavior of keratinocytes. Collectively, these results indicate that a desmosomal molecule, PG, is capable of regulating single cell motility through matrix deposition in concert with Rho GTPases, independently of its role as a cell-cell adhesion molecule. Results PG regulates keratinocyte cell polarity and single-cell ...

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“…46,47 Accumulating evidence suggests that cytosolic NME/NDPKs NME1 but also often NME2, interact with and affect different components and regulators of the cytoskeleton, including actin-binding proteins, intermediate filaments, and cytoskeleton attachment structures (adherens junctions, desmosomes, and focal adhesions) in cells from a variety of organisms and tissues, and in the course of development, suggesting that this association is evolutionarily conserved and may serve an essential function. [48][49][50][51][52][53][54][55] The interactions of NDPK with components of the cytoskeletal machinery are highly relevant, given the well-established role of the cytoskeleton in cell motility, a critical determinant of the metastasis process. NME1 has also been reported to bind proteins belonging to small and heterotrimeric G-proteins ( [56][57][58][59][60][61] ; and Filic 62 upcoming issue; Abu-Taha et al, 63 this issue), transcriptional complexes ( 64-69 ; Sharma et al, 70 Pandey and Robertson, 71 and Puts et al, 72 all in this issue), and components of signaling pathways of MAPK, [73][74][75] TGF-β [76][77][78] and Notch, 79 as well as other factors promoting invasion and metastasis ( 80,81 ; Ferrucci et al 82 upcoming issue).…”

Section: Nme In Metastasismentioning

confidence: 99%

The NDPK/NME superfamily: state of the art

Boissan

Schlattner

Lacombe

2018

Laboratory Investigation

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Nucleoside diphosphate kinases (NDPK) are nucleotide metabolism enzymes encoded by NME genes (also called NM23). Given the fact that not all NME-encoded proteins are catalytically active NDPKs and that NM23 generally refers to clinical studies on metastasis, we use here NME/NDPK to denote the proteins. Since their discovery in the 1950's, NMEs/NDPKs have been shown to be involved in multiple physiological and pathological cellular processes, but the molecular mechanisms have not been fully determined. Recent progress in elucidating these underlying mechanisms has been presented by experts in the field at the 10th International Congress on the NDPK/NME/AWD protein family in October 2016 in Dubrovnik, Croatia, and is summarized in review articles or original research in this and an upcoming issue of Laboratory Investigation. Within this editorial, we discuss three major cellular processes that involve members of the multi-functional NME/NDPK family: (i) cancer and metastasis dissemination, (ii) membrane remodeling and nucleotide channeling, and iii) protein histidine phosphorylation.

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Plakoglobin interacts with and increases the protein levels of metastasis suppressor Nm23-H2 and regulates the expression of Nm23-H1

Cited by 52 publications

References 68 publications

An EMMPRIN/γ-catenin/Nm23 complex drives ATP production and actomyosin contractility at endothelial junctions

An EMMPRIN/γ-catenin/Nm23 complex drives ATP production and actomyosin contractility at endothelial junctions

Plakoglobin regulates cell motility through Rho- and fibronectin-dependent Src signaling

The NDPK/NME superfamily: state of the art

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