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

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241

The PIP5K family Three isoforms of PIP5K have been identified and are known as PIP5K, PIP5K and PIP5K (Ishihara et al., 1996;Loijens and Anderson, 1996;Oude Weernink et al., 2004b). PIP5K and PIP5K each have a molecular mass of 64 kDa. Mouse PIP5K has three different splice variants of 69 or 72 kDa in size (Box 1). The nomenclature of PIP5K isoforms has become somewhat confusing because the nomenclature for mouse genes is opposite to that of human genes (human PIP5K is similar to mouse PIP5K and vice versa). In addition, several synonyms are currently in use for this protein family, including PI5PK, PIPK1, PI5PK1 and PIPkin. Here, we use the term PIP5K for this family together with the isoform nomenclature that is used for the human proteins, because this terminology is now used by the National Centre for Bioinformatics (NCBI) (Box 1). Further variation in the sequence of PIP5Ks is created through the generation of splice variants. In mice, eight , two  and three  splice variants have been described in the Ensemble database, whereas for humans three , four  and It has long been known that phosphoinositides are present in cellular membranes, but only in the past four decades has our understanding of their importance for proper cell function advanced significantly. Key to determining the biological roles of phosphoinositides is understanding the enzymes involved in their metabolism. Although many such enzymes have now been identified, there is still much to learn about their cellular functions. Phosphatidylinositol 4-phosphate 5-kinases (PIP5Ks) are a group of kinases that catalyse the production of phosphatidylinositol (4,5)-bisphosphate [PtdIns(4,5)P 2 ]. As well as being a substrate for the enzymes phospholipase C (PLC) and phosphatidylinositol 3-kinase (PI3K), PtdIns(4,5)P 2 acts as a second messenger in its own right, influencing a variety of cellular processes. In this Commentary, we review how PIP5Ks are modulated to achieve regulated PtdIns(4,5)P 2 production, and discuss the role of these proteins in different cellular processes.

Section: Cellular Functions Of Pip5ksmentioning

confidence: 99%

Section: Cellular Functions Of Pip5ksmentioning

confidence: 99%

PIP5K-driven PtdIns(4,5)P2 synthesis: regulation and cellular functions

Bout

Divecha

2009

266

241

“…mAbp1 was PCR amplified from GFP-mAbp1 and GFP-mAbp1(W415K) (Cortesio et al, 2010) using a forward primer containing an EcoRI site, 59-GTC ACG GAA TTC GAT GGC GGT GAA CCT GAG CCG GAA C-39 and BamHIcontaining reverse primer, 59-CGA TCG CGG ATC CTC ACT CTA TGA GCT CCA CGT AGT TGG CAG G-39. PCR-amplified mAbp1 and mAbp1(W415K) was cloned into the EcoRI and BamHI sites of pmCherry-C1 (Lokuta et al, 2007). mCherry-C1-mAbp1 and mCherry-C1-Abp(W415K) were subcloned into pMXIres-GFP vector (Clive Svendsen, University of Wisconsin, Madison, WI) with the Ires-GFP portion excised.…”

Section: Dna and Sirna Constructsmentioning

confidence: 99%

Src-mediated phosphorylation of mammalian Abp1 (DBNL) regulates podosome rosette formation in transformed fibroblasts

Boateng

Cortesio

Huttenlocher

2012

Self Cite

There were errors published in J. Cell Sci. 125, 1329-1341.All mentions of Tyr340 and Tyr350 should read Tyr337 and Tyr347, respectively.In addition, the double phospho-mutant should be mCherry-mAbp1(Y337E,Y347F).The corrected legend to Fig. 9 appears below. Fig. 9. Model of mAbp1 regulation of podosome formation and invasive migration. mAbp1 binds to filamentous actin and is phosphorylated by Src at Y337 and Y347 in the proline-rich region (oval). Phosphorylation of mAbp1 at Y347 is required for podosome rosette formation and the inhibition of invasive migration. Y347 might be the crucial residue that mediates maturation of podosome dots to rosettes. Conversely, Src phosphorylation of both Y337 and Y347 impairs formation of podosome dots.We apologise for these errors. Summary Podosomes are dynamic actin-based structures that mediate adhesion to the extracellular matrix and localize matrix degradation to facilitate cell motility and invasion. Drebrin-like protein (DBNL), which is homologous to yeast mAbp1 and is therefore known as mammalian actin-binding protein 1 (mAbp1), has been implicated in receptor-mediated endocytosis, vesicle recycling and dorsal ruffle formation. However, it is not known whether mAbp1 regulates podosome formation or cell invasion. In this study, we found that mAbp1 localizes to podosomes and is necessary for the formation of podosome rosettes in Src-transformed fibroblasts. Despite their structural similarity, mAbp1 and cortactin play distinct roles in podosome regulation. Cortactin was necessary for the formation of podosome dots, whereas mAbp1 was necessary for the formation of organized podosome rosettes in Src-transformed cells. We identified specific Src phosphorylation sites, Tyr337 and Tyr347 of mAbp1, which mediate the formation of podosome rosettes and degradation of the ECM. In contrast to dorsal ruffles, the interaction of mAbp1 with WASP-interacting protein (WIP) was not necessary for the formation of podosome rosettes. Finally, we showed that depletion of mAbp1 increased invasive cell migration, suggesting that mAbp1 differentially regulates matrix degradation and cell invasion. Collectively, our findings identify a role for mAbp1 in podosome rosette formation and cell invasion downstream of Src.

“…We suggest that activation of PIP5K and increased local synthesis of PtdIns(4,5)P 2 at the trailing edge of a migrating cell regulates vinculin interactions, to decrease focal adhesion stability. Interestingly, a recent study has demonstrated that PIP5K is localised to the uropod and that PtdIns(4,5)P 2 synthesis is required for uropod retraction during neutrophil migration (Lokuta et al, 2007).…”

Section: E61lmentioning

confidence: 99%

Rac controls PIP5K localisation and PtdIns(4,5)P2 synthesis, which modulates vinculin localisation and neurite dynamics

Halstead

Savaskan

Bout

et al. 2010

SummaryIn N1E-115 cells, neurite retraction induced by neurite remodelling factors such as lysophosphatidic acid, sphingosine 1-phosphate and semaphorin 3A require the activity of phosphatidylinositol 4-phosphate 5-kinases (PIP5Ks). PIP5Ks synthesise the phosphoinositide lipid second messenger phosphatidylinositol(4,5)bisphosphate [PtdIns(4,5)P 2 ], and overexpression of active PIP5K is sufficient to induce neurite retraction in both N1E-115 cells and cerebellar granule neurones. However, how PIP5Ks are regulated or how they induce neurite retraction is not well defined. Here, we show that neurite retraction induced by PIP5K is dependent on its interaction with the low molecular weight G protein Rac. We identified the interaction site between PIP5K and Rac1 and generated a point mutant of PIP5K that no longer interacts with endogenous Rac. Using this mutant, we show that Rac controls the plasma membrane localisation of PIP5K and thereby the localised synthesis of PtdIns(4,5)P 2 required to induce neurite retraction. Mutation of this residue in other PIP5K isoforms also attenuates their ability to induce neurite retraction and to localise at the membrane. To clarify how increased levels of PtdIns(4,5)P 2 induce neurite retraction, we show that mutants of vinculin that are unable to interact with PtdIns(4,5)P 2 , attenuate PIP5K-and LPA-induced neurite retraction. Our findings support a role for PtdIns(4,5)P 2 synthesis in the regulation of vinculin localisation at focal complexes and ultimately in the regulation of neurite dynamics.