Asymmetric Localization of Calpain 2 during Neutrophil Chemotaxis

Nuzzi, Paul A.; Senetar, Melissa A.; Huttenlocher, Anna

doi:10.1091/mbc.e06-09-0876

Cited by 47 publications

(47 citation statements)

References 62 publications

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“…Syndecan-translocation to lipid rafts plays a role in cell migration (39). Lipid rafts are known to serve as platforms for molecules (42), and translocation of molecules, such as ICAM-1 (30), calpain (32), and integrins (25), to lipid rafts is necessary to activate cell migration. We demonstrated that Epac increased translocation of syndecan-2 to lipid rafts.…”

Section: Discussionmentioning

confidence: 99%

“…2B) or the expression of the other HSPGs (data not shown). Since syndecan is known to translocate to lipid rafts (40), which serve as platforms for molecules involved in cell migration (26,30,32), we hypothesized that such large particle size indicates accumulation of syndecan-2 in lipid rafts. Indeed, immunocytochemistry showed that both Epac agonist and Epac1 overexpression increased colocalization of syndecan-2 with lipid rafts.…”

Section: Epac Increases Migration In Melanomamentioning

confidence: 99%

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Epac increases melanoma cell migration by a heparan sulfate-related mechanism

Baljinnyam

Iwatsubo

Kurotani

et al. 2009

American Journal of Physiology-Cell Physiology

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2009.-Melanoma, the most malignant form of human skin cancer, has a poor prognosis due to its strong metastatic ability. It was recently demonstrated that Epac, an effector molecule of cAMP, is involved in regulating cell migration; however, the role of Epac in melanoma cell migration remains unclear. We thus examined whether Epac regulates cell migration and metastasis of melanoma. Epac activation, by either specific agonist or overexpression of Epac, increased melanoma cell migration. Deletion of endogenous Epac with small interfering RNA decreased basal melanoma cell migration. These data suggested a major role of Epac in melanoma cell migration. Epac-induced cell migration was mediated by translocation of syndecan-2, a cell-surface heparan sulfate proteoglycan, to lipid rafts. This syndecan-2 translocation was regulated by tubulin polymerization via the Epac/phosphoinositol-3 kinase pathway. Epacinduced cell migration was also regulated by the production of heparan sulfate, a major extracellular matrix. Epac-induced heparan sulfate production was attributable to the increased expression of N-deacetylase/N-sulfotransferase-1 (NDST-1) accompanied by an increased NDST-1 translation rate. Finally, Epac overexpression enhanced lung colonization of melanoma cells in mice. Taken together, these data indicate that Epac regulates melanoma cell migration/ metastasis mostly via syndecan-2 translocation and heparan sulfate production. metastasis; phosphoinositol-3 kinase; N-deacetylase/N-sulfotransferase-1

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Section: Discussionmentioning

confidence: 99%

Section: Epac Increases Migration In Melanomamentioning

confidence: 99%

Epac increases melanoma cell migration by a heparan sulfate-related mechanism

Baljinnyam

Iwatsubo

Kurotani

et al. 2009

American Journal of Physiology-Cell Physiology

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“…HL-60 cells (UCSF tissue culture facility) were cultured and differentiated as previously described (Nuzzi et al, 2007b). Phoenix viral packaging cells were transiently transfected by calcium-phosphate precipitation (Nuzzi et al, 2007a).…”

Section: Cell Culture and Retroviral Infectionmentioning

confidence: 99%

“…Primary human neutrophils, undifferentiated and differentiated HL-60 cells, and HEK 293 cells were lysed (Nuzzi et al, 2007b), samples were clarified by centrifugation, and protein concentration was determined using a bicinchoninic acid (BCA) protein assay (Pierce, Rockford, IL). Equal amounts of total protein were denatured in SDS sample buffer, resolved on 4 -20% gradient Representative images of neutrophils demonstrate localization of endogenous PIPKI␥ (P␥; C) and active RhoA (rhotekin; D) to the cell rear upon fMLP stimulation.…”

Section: Protein Extraction Antibodies and Immunoblotsmentioning

confidence: 99%

Type Iγ PIP Kinase Is a Novel Uropod Component that Regulates Rear Retraction during Neutrophil Chemotaxis

Lokuta

Senetar²,

Bennin

et al. 2007

MBoC

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Cell polarization is necessary for directed migration and leukocyte recruitment to inflamed tissues. Recent progress has been made in defining the molecular mechanisms that regulate chemoattractant-induced cell polarity during chemotaxis, including the contribution of phosphoinositide 3-kinase (PI3K)-dependent phosphatidylinositol (3,4,5)-trisphosphate [PtdIns(3,4,5)P 3 ] synthesis at the leading edge. However, less is known about the molecular composition of the cell rear and how the uropod functions during cell motility. Here, we demonstrate that phosphatidylinositol phosphate kinase type I␥ (PIPKI␥661), which generates PtdIns(4,5)P 2 , is enriched in the uropod during chemotaxis of primary neutrophils and differentiated HL-60 cells (dHL-60). Using time-lapse microscopy, we show that enrichment of PIPKI␥661 at the cell rear occurs early upon chemoattractant stimulation and is persistent during chemotaxis. Accordingly, we were able to detect enrichment of PtdIns(4,5)P 2 at the uropod during chemotaxis. Overexpression of kinase-dead PIPKI␥661 compromised uropod formation and rear retraction similar to inhibition of ROCK signaling, suggesting that PtdIns(4,5)P 2 synthesis is important to elicit the backness response during chemotaxis. Together, our findings identify a previously unknown function for PIPKI␥661 as a novel component of the backness signal that regulates rear retraction during chemotaxis.

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“…During neutrophil migration, actin microfi lament polymerization leads to the extension of membrane projections (i.e., protrusions) at the leading edge, including fi lopodia and lamellipodia, which are required for directional migration. In the case of neutrophils, exposure to a chemoattractant gradient induces the rapid enrichment of the protease calpain 2 at the leading edge where it colocalizes with F-actin (Nuzzi et al, 2007). Localization of the protease at the leading edge seems to be causal for neutrophil migration because the expression of an inactive protease variant (Calpain PD) generates multiple lamellipodia surrounding neutrophils without a defi ned leading edge and prevents effi cient chemotaxis (Nuzzi et al, 2007).…”

Section: Role Of Calpain In Polarization During Cell Migrationmentioning

confidence: 99%

Regulation of cell polarity by controlled proteolytic systems

Bórquez¹,

González-Billault²

2011

Biol. Res.

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Epithelial and neuronal cells are highly asymmetric, with discrete regions responsible for different roles that underlie the generation of specifi c compartments within cells that are distinct in biochemical composition, structure, and morphology that ultimately lead to distinct functions. Controlled and specifi c molecular targeting and sorting have been studied to understand the generation of asymmetric domains inside cells. Recently, a new and complementary explanation has emerged to account for the generation of domains that are enriched by a subset of proteins or polarization determinants: local proteolysis. In this review, we discuss the most conspicuous proteolytic systems that may contribute to the generation of cell polarity, namely the ubiquitin-proteosome and the calpain systems. Specifi cally, we focus this review on two cellular processes that depend on the acquisition of cell polarity; cell migration and the establishment of an axon in a neuronal cell.

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Asymmetric Localization of Calpain 2 during Neutrophil Chemotaxis

Cited by 47 publications

References 62 publications

Epac increases melanoma cell migration by a heparan sulfate-related mechanism

Epac increases melanoma cell migration by a heparan sulfate-related mechanism

Type Iγ PIP Kinase Is a Novel Uropod Component that Regulates Rear Retraction during Neutrophil Chemotaxis

Regulation of cell polarity by controlled proteolytic systems

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