Quantitative and Dynamic Assessment of the Contribution of the ER to Phagosome Formation

Touret, Nicolas; Paroutis, Paul; Terebiznik, Mauricio R.; Harrison, Rene E.; Trombetta, Sergio; Pypaert, Marc; Chow, Amy; Jiang, Aimin; Shaw, James E.; Yip, Christopher M.; Moore, Hsiao-Ping; Wel, Nicole N. van der; Houben, Diane; Peters, Peter J.; Chastellier, Chantal de; Mellman, Ira; Grinstein, Sergio

doi:10.1016/j.cell.2005.08.018

Cited by 251 publications

(223 citation statements)

References 59 publications

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“…Confocal microscopy has shown that internal membranes within the cell fuse with plasma membrane during the course of particle ingestion, and that recycling endosomes are the primary source of membrane for enlargement of phagocytic cup [22]. Flow cytometric assessment of particle engulfment has to some extent replaced microscopic observation [23] particularly as the kinetics of uptake of fluorescent targets by phagocytes can be followed by instruments capable of time-resolved measurements in a stirred cuvette at 37°C [24].…”

Section: Flow Cytometric Assay Of Phagocytosismentioning

confidence: 99%

A new role for the P2X7 receptor: a scavenger receptor for bacteria and apoptotic cells in the absence of serum and extracellular ATP

Wiley

2012

Purinergic Signalling

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The P2X7 receptor is widely recognized to mediate the proinflammatory effects of extracellular ATP. However this receptor in the absence of ATP may have a function unrelated to inflammation. Our data show that P2X7 expressed on the surface of monocyte/macrophages or on epithelial HEK-293 cells greatly augments the engulfment of latex beads and live and heat-killed bacteria by effector phagocyte in the absence of ATP and serum. The expression of P2X7 on the effector also confers the ability to phagocytose apoptotic target cells and an accumulation of P2X7 can be seen at the attachment point to the target. Activation of the P2X7 receptor by ATP causes a slow dissociation (over 10-15 min) of nonmuscle myosin from the P2X7 membrane complex and abolishes further P2X7-mediated phagocytosis of these targets. The recent crystal structure of the homologous zebrafish P2X4 receptor shows an exposed "nose" of the ectodomain (residues 115-162) which contains three of the five disulfide bonds conserved in all P2X receptors. Three short biotin-labeled peptides mimicking sequence of this exposed region bound to apoptotic target cells but not to either viable cells or to other target particles. All three peptides contained one or two cysteine residues and their replacement by alanine abolished peptide binding. These data implicate thiol-disulfide exchange reactions in the initial tethering of apoptotic cells to macrophage and establish P2X7 as one of the scavenger receptors involved in the recognition and removal of apoptotic cells in the absence of extracellular ATP and serum.

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Section: Flow Cytometric Assay Of Phagocytosismentioning

confidence: 99%

A new role for the P2X7 receptor: a scavenger receptor for bacteria and apoptotic cells in the absence of serum and extracellular ATP

Wiley

2012

Purinergic Signalling

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“…Other studies suggested the existence of endoplasmic reticulum (ER)-mediated phagocytosis (8 -10), whereby the ER membrane was targeted to the phagocytic site to aid in phagosome formation. However, by using a combination of biochemical, fluorescence imaging and electron microscopy techniques, Grinstein and colleagues (11) did not obtain evidence to prove the direct fusion between the ER and the plasma membrane. ER-mediated phagocytosis remains a subject of controversy.…”

Section: Vesicle-associated Membrane Protein-8/endobrevin Negativelymentioning

confidence: 99%

Vesicle-Associated Membrane Protein-8/Endobrevin Negatively Regulates Phagocytosis of Bacteria in Dendritic Cells

Cai

Wang

et al. 2008

The Journal of Immunology

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Phagocytosis is a specialized mechanism used by mammalian cells, particularly the cells of the immune system, such as dendritic cells (DC) and macrophages, to protect the host against infection. The process involves a complex cascade of pathways, from the ligation of surface receptors of phagocytes with components of the microorganism’s surface, formation of phagosomes and subsequently phagolysosomes, to the eventual presentation of foreign Ags. Vesicle-associated membrane protein (VAMP)-8/endobrevin has been shown previously to function in the endocytic pathways. Our results showed that VAMP-8 colocalized with lysosome-associated membrane protein-2, and a significant amount of VAMP-8 was recruited to the phagosomes during bacterial ingestion. However, overexpression of VAMP-8 significantly inhibited phagocytosis in DC. We also found that the phagocytic activity of VAMP-8−/− DC was significantly higher than wild-type VAMP-8+/+ DC, thus further confirming that VAMP-8 negatively regulates phagocytosis in immature DC.

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“…Mais la majeure partie de l'attention portée à ce modèle était due à sa capacité d'expliquer le mécanisme mal compris de la présentation croisée des antigènes [4,5]. La participation du RE dans la formation du phagosome a été récemment ré-examinée en utilisant diverses approches biophysiques et biochimiques [6]. Une quantification des composants du phagosome présents au cours de sa formation par microscopie de fluorescence ou électronique, et par une approche biochimique intégrative, n'a indiqué aucune contribution significative du RE.…”

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Caractéristiques dynamiques et fonctionnelles de la membrane du phagosome

Touret

Grinstein

2006

Med Sci (Paris)

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Quantitative and Dynamic Assessment of the Contribution of the ER to Phagosome Formation

Cited by 251 publications

References 59 publications

A new role for the P2X7 receptor: a scavenger receptor for bacteria and apoptotic cells in the absence of serum and extracellular ATP

A new role for the P2X7 receptor: a scavenger receptor for bacteria and apoptotic cells in the absence of serum and extracellular ATP

Vesicle-Associated Membrane Protein-8/Endobrevin Negatively Regulates Phagocytosis of Bacteria in Dendritic Cells

Caractéristiques dynamiques et fonctionnelles de la membrane du phagosome

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