PTP1B Dephosphorylates N-Ethylmaleimide-sensitive Factor and Elicits SNARE Complex Disassembly during Human Sperm Exocytosis

Zarelli, Valeria E.P.; Ruete, María Celeste; Roggero, Carlos M.; Mayorga, Luis S.; Tomes, Claudia N.

doi:10.1074/jbc.m807614200

Cited by 48 publications

(60 citation statements)

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“…Zona binding evokes Ca 2+ entry (see Section 5.3.1) and this causes both the dissociation of the MUPP1/CaMKII fusion clamp [64] and a calcineurin-mediated dephosphorylation of synaptotagmin VI [63]. The dephosphorylation of synaptotagmins also appear to be essential for the acrosome reaction [59, 62,117,63] (unpublished observation). The role of Rab3A [62] and Rab2A (unpublished observation) in the formation of the cis ternary SNARE complex conformation is not yet clear.…”

Section: Fig 52 Two Step Model For Snare Mediated Acrosome Exocytosmentioning

confidence: 99%

Membrane Fusions During Mammalian Fertilization

Gadella

Evans

2011

Advances in Experimental Medicine and Biology

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Successful completion of fertilization in mammals requires three different types of membrane fusion events. Firstly, the sperm cell will need to secrete its acrosome contents (acrosome exocytosis; also known as the acrosome reaction); this allows the sperm to penetrate the extracellular matrix of the oocyte (zona pellucida) and to reach the oocyte plasma membrane, the site of fertilization. Next the sperm cell will bind and fuse with the oocyte plasma membrane (also known as the oolemma), which is a different type of fusion in which two different cells fuse together. Finally, the fertilized oocyte needs to prevent polyspermic fertilization, or fertilization by more than one sperm. To this end, the oocyte secretes the contents of cortical granules by exocytotic fusions of these vesicles with the oocyte plasma membrane over the entire oocyte cell surface (also known as the cortical reaction or cortical granule exocytosis). The secreted cortical contents modify the zona pellucida, converting it to a state that is unreceptive to sperm, constituting a block to polyspermy. In addition, there is a block at the level of the oolemma (also known as the membrane block to polyspermy). IntroductionFertilization of the oocyte involves three membrane fusion events [1] namely, (1) a preparative series of secretion membrane fusions at the apical sperm surface known as acrosome exocytosis [2]. The membrane fusions are induced when the sperm cell binds to specific zona binding proteins at the sperm surface [3][4][5][6][7]. The acrosome exocytosis is a multipoint membrane fusion event between the sperm plasma membrane and the outer acrosomal membrane (see Fig. 5.1 [8,9]) and the exposed acrosomal content is required for sperm to penetrate the zona pellucida [10][11][12]. This so-called zona drilling effectively takes place because the sperm at this stage also has acquired hyperactivated motility [13]. (2) After zona penetration the sperm enters the perivitelline space where it can bind and fuse with the oocyte plasma membrane [14,15]. This is the actual fertilization fusion in which the contents of the sperm are delivered into the oocyte cytoplasm. The plasma membrane of the equatorial segment (see Fig. 5.1) is the site where proteins are located that orchestrate sperm-oocyte binding and fusion [16]. (3) In order to prevent polyspermy the oocyte has to activate defense systems to block redundant sperm-oocyte fusion [17]. To this end the first fertilizing sperm delivers activation factors

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Section: Fig 52 Two Step Model For Snare Mediated Acrosome Exocytosmentioning

confidence: 99%

Membrane Fusions During Mammalian Fertilization

Gadella

Evans

2011

Advances in Experimental Medicine and Biology

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“…Recently, the ATPase NSF was identified as a substrate for PTP1B (42). NSF activity is tightly modulated by its phosphorylation status; dephosphorylation promotes its interaction with endosomal components and results in endosome fusion.…”

Section: Discussionmentioning

confidence: 99%

“…PTP-MEG2 is located on the cytoplasmic face of secretory vesicles where it regulates vesicle size by promoting homotypic vesicle fusion via tyrosine dephosphorylation of NSF (41). Recently, PTP1B has been identified as a PTP that dephosphorylates NSF in acrosomes (42). Additionally, PTP1B has been implicated in the dephosphorylation and inactivation of internalized RTKs, including Met and EGFR (26,30), and in MVB maturation in response to EGF (39).…”

Section: Signaling Via Receptor Tyrosine Kinases (Rtks)mentioning

confidence: 99%

“…After vesicle fusion, the SNARE complex, which includes ␣-soluble N-ethylmaleimide-sensitive factor (NSF)-associated protein (␣-SNAP), must be disassembled via ATP hydrolysis of its ␣-SNAP subunit by the NSF; inefficient disassembly of the SNARE complex halts further vesicle fusion. The activity of NSF is regulated via its phosphorylation status; the kinases Fes and Ca 2ϩ /calmodulin-dependent protein kinase II (40) and the phosphatases PTP-MEG2 (41) and PTP1B (42) have been shown to control NSF phosphorylation. PTP-MEG2 is located on the cytoplasmic face of secretory vesicles where it regulates vesicle size by promoting homotypic vesicle fusion via tyrosine dephosphorylation of NSF (41).…”

Section: Signaling Via Receptor Tyrosine Kinases (Rtks)mentioning

confidence: 99%

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Protein-tyrosine Phosphatase 1B Modulates Early Endosome Fusion and Trafficking of Met and Epidermal Growth Factor Receptors

Sangwan

Abella

Lai

et al. 2011

Journal of Biological Chemistry

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Background:Signaling from RTKs is regulated at multiple levels; however, the role played by dephosphorylation in this process remains poorly understood. Results: We show that loss of PTP1B activity leads to abrogated receptor trafficking via the endocytic pathway. Conclusion: Dephosphorylation of the vesicle fusion machinery component NSF by PTP1B is required for RTK trafficking. Significance: This identifies a novel mechanism through which PTP1B can modulate RTK signaling.

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“…This has facilitated the functional study of individual proteins as targets of particular protein kinases, whilst uncovering the significance of phosphorylation/dephosphorylation events in the regulation of exocytosis, such as in: synaptic transmission and cell plasticity (Amin, et al, 2008;Barclay, et al, 2003;Boczan, et al, 2004), neuronal morphogenesis (Chernyshova, et al, 2011), insulin secretion (Butelman, 1990;Sugawara, et al, 2009;Wang & Thurmond, 2010), insulin stimulated GLUT4 transport (Aran, et al, 2011;X. W. Chen, et al, 2011a;Sano, et al, 2011), mast cell and platelet degranulation (Fitzgerald & Reed, 1999;Foger, et al, 2011), exocytosis of factors required for neutrophil adhesion (Fu, et al, 2005), acrosomal exocytosis in sperm (Castillo Bennett, et al, 2010;Zarelli, et al, 2009) and lung surfactant exocytosis (Gerelsaikhan, et al, 2011). It has now become obvious that phospho-regulation of exocytosis is a complex and dynamic process implicated at almost all points along the exocytic route, from recruitment and transport of vesicles to their ultimate fusion at the plasma membrane ( Figure 1&2).…”

Section: Phosphorylation As a Means Of Controlling Protein Activitymentioning

confidence: 99%