NADPH oxidase is internalized by clathrin-coated pits and localizes to a Rab27A/B GTPase-regulated secretory compartment in activated macrophages

Patrick Ejlerskov; Dan Ploug Christensen; David Beyaie; James B Burritt; Marie-Helene Paclet; Agnes Gorlach; Bo van Deurs; Frederik Vilhardt

doi:10.1074/jbc.M111.293696

NADPH oxidase is internalized by clathrin-coated pits and localizes to a Rab27A/B GTPase-regulated secretory compartment in activated macrophages

Patrick Ejlerskov, Dan Ploug Christensen, David Beyaie, James B Burritt, Marie-Helene Paclet, Agnes Gorlach, Bo van Deurs, Frederik Vilhardt

20 Citationer (Scopus)

Abstract

Here, we report that activation of different types of tissue macrophages, including microglia, by lipopolysaccharide (LPS) or GM-CSF stimulation correlates with the quantitative redistribution of NADPH oxidase (cyt b ₅₅₈) from the plasma membrane to an intracellular stimulus-responsive storage compartment. Cryo-immunogold labeling of gp91 ^phox and CeCl ₃cytochemistry showed the presence of gp91 ^phox and oxidant production in numerous small (<100 nm) vesicles. Cell homogenization and sucrose gradient centrifugation in combination with transferrin-HRP/DAB ablation showed that more than half of cyt b ₅₅₈ is present in fractions devoid of endosomal markers, which is supported by morphological evidence to show that the cyt b ₅₅₈-containing compartment is distinct from endosomes or biosynthetic organelles. Streptolysin-O-mediated guanosine 5′-3-O-(thio)triphosphate loading of Ra2 microglia caused exocytosis of a major complement of cyt b ₅₅₈ under conditions where lysosomes or endosomes were not mobilized. We establish phagocytic particles and soluble mediators ATP,TNFα, and CD40L as physiological inducers of cyt b ₅₅₈ exocytosis to the cell surface, and by shRNA knockdown, we identify Rab27A/B as positive or negative regulators of vesicular mobilization to the phagosome or the cell surface, respectively. Exocytosis was followed by clathrin-dependent internalization of cyt b ₅₅₈, which could be blocked by a dominant negative mutant of the clathrin-coated pit-associated protein Eps15. Re-internalized cyt b ₅₅₈ did not reach lysosomes but associated with recycling endosomes and undefined vesicular elements. In conclusion, cyt b ₅₅₈depends on clathrin for internalization, and in activated macrophages NADPH oxidase occupies a Rab27A/B-regulated secretory compartment, which allows rapid agonist-induced redistribution of superoxide production in the cell.

Originalsprog	Engelsk
Tidsskrift	Journal of Biological Chemistry
Vol/bind	287
Udgave nummer	7
Sider (fra-til)	4835-52
Antal sider	18
ISSN	0021-9258
DOI	https://doi.org/10.1074/jbc.M111.293696
Status	Udgivet - 10 feb. 2012

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10.1074/jbc.M111.293696

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NADPH oxidase is internalized by clathrin-coated pits and localizes to a Rab27A/B GTPase-regulated secretory compartment in activated macrophages. / Ejlerskov, Patrick; Christensen, Dan Ploug; Beyaie, David et al.

I: Journal of Biological Chemistry, Bind 287, Nr. 7, 10.02.2012, s. 4835-52.

Publikation: Bidrag til tidsskrift › Tidsskriftartikel › Forskning › peer review

@article{99b3fb08a57241fea208a1bd4dead673,

title = "NADPH oxidase is internalized by clathrin-coated pits and localizes to a Rab27A/B GTPase-regulated secretory compartment in activated macrophages",

abstract = "Here, we report that activation of different types of tissue macrophages, including microglia, by lipopolysaccharide (LPS) or GM-CSF stimulation correlates with the quantitative redistribution of NADPH oxidase (cyt b 558) from the plasma membrane to an intracellular stimulus-responsive storage compartment. Cryo-immunogold labeling of gp91 phox and CeCl 3cytochemistry showed the presence of gp91 phox and oxidant production in numerous small (<100 nm) vesicles. Cell homogenization and sucrose gradient centrifugation in combination with transferrin-HRP/DAB ablation showed that more than half of cyt b 558 is present in fractions devoid of endosomal markers, which is supported by morphological evidence to show that the cyt b 558-containing compartment is distinct from endosomes or biosynthetic organelles. Streptolysin-O-mediated guanosine 5′-3-O-(thio)triphosphate loading of Ra2 microglia caused exocytosis of a major complement of cyt b 558 under conditions where lysosomes or endosomes were not mobilized. We establish phagocytic particles and soluble mediators ATP,TNFα, and CD40L as physiological inducers of cyt b 558 exocytosis to the cell surface, and by shRNA knockdown, we identify Rab27A/B as positive or negative regulators of vesicular mobilization to the phagosome or the cell surface, respectively. Exocytosis was followed by clathrin-dependent internalization of cyt b 558, which could be blocked by a dominant negative mutant of the clathrin-coated pit-associated protein Eps15. Re-internalized cyt b 558 did not reach lysosomes but associated with recycling endosomes and undefined vesicular elements. In conclusion, cyt b 558depends on clathrin for internalization, and in activated macrophages NADPH oxidase occupies a Rab27A/B-regulated secretory compartment, which allows rapid agonist-induced redistribution of superoxide production in the cell.",

keywords = "Adenosine Triphosphate, Animals, CD40 Ligand, Calcium-Binding Proteins, Cells, Cultured, Clathrin, Clathrin-Coated Vesicles, Cytochrome b Group, Endosomes, Exocytosis, Intracellular Signaling Peptides and Proteins, Macrophage Activation, Macrophages, Membrane Glycoproteins, Microglia, NADPH Oxidase, Rats, Superoxides, Tumor Necrosis Factor-alpha, rab GTP-Binding Proteins",

author = "Patrick Ejlerskov and Christensen, {Dan Ploug} and David Beyaie and Burritt, {James B} and Marie-Helene Paclet and Agnes Gorlach and {van Deurs}, Bo and Frederik Vilhardt",

year = "2012",

month = feb,

day = "10",

doi = "10.1074/jbc.M111.293696",

language = "English",

volume = "287",

pages = "4835--52",

journal = "Journal of Biological Chemistry",

issn = "0021-9258",

publisher = "American Society for Biochemistry and Molecular Biology, Inc.",

number = "7",

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TY - JOUR

T1 - NADPH oxidase is internalized by clathrin-coated pits and localizes to a Rab27A/B GTPase-regulated secretory compartment in activated macrophages

AU - Ejlerskov, Patrick

AU - Christensen, Dan Ploug

AU - Beyaie, David

AU - Burritt, James B

AU - Paclet, Marie-Helene

AU - Gorlach, Agnes

AU - van Deurs, Bo

AU - Vilhardt, Frederik

PY - 2012/2/10

Y1 - 2012/2/10

N2 - Here, we report that activation of different types of tissue macrophages, including microglia, by lipopolysaccharide (LPS) or GM-CSF stimulation correlates with the quantitative redistribution of NADPH oxidase (cyt b 558) from the plasma membrane to an intracellular stimulus-responsive storage compartment. Cryo-immunogold labeling of gp91 phox and CeCl 3cytochemistry showed the presence of gp91 phox and oxidant production in numerous small (<100 nm) vesicles. Cell homogenization and sucrose gradient centrifugation in combination with transferrin-HRP/DAB ablation showed that more than half of cyt b 558 is present in fractions devoid of endosomal markers, which is supported by morphological evidence to show that the cyt b 558-containing compartment is distinct from endosomes or biosynthetic organelles. Streptolysin-O-mediated guanosine 5′-3-O-(thio)triphosphate loading of Ra2 microglia caused exocytosis of a major complement of cyt b 558 under conditions where lysosomes or endosomes were not mobilized. We establish phagocytic particles and soluble mediators ATP,TNFα, and CD40L as physiological inducers of cyt b 558 exocytosis to the cell surface, and by shRNA knockdown, we identify Rab27A/B as positive or negative regulators of vesicular mobilization to the phagosome or the cell surface, respectively. Exocytosis was followed by clathrin-dependent internalization of cyt b 558, which could be blocked by a dominant negative mutant of the clathrin-coated pit-associated protein Eps15. Re-internalized cyt b 558 did not reach lysosomes but associated with recycling endosomes and undefined vesicular elements. In conclusion, cyt b 558depends on clathrin for internalization, and in activated macrophages NADPH oxidase occupies a Rab27A/B-regulated secretory compartment, which allows rapid agonist-induced redistribution of superoxide production in the cell.

AB - Here, we report that activation of different types of tissue macrophages, including microglia, by lipopolysaccharide (LPS) or GM-CSF stimulation correlates with the quantitative redistribution of NADPH oxidase (cyt b 558) from the plasma membrane to an intracellular stimulus-responsive storage compartment. Cryo-immunogold labeling of gp91 phox and CeCl 3cytochemistry showed the presence of gp91 phox and oxidant production in numerous small (<100 nm) vesicles. Cell homogenization and sucrose gradient centrifugation in combination with transferrin-HRP/DAB ablation showed that more than half of cyt b 558 is present in fractions devoid of endosomal markers, which is supported by morphological evidence to show that the cyt b 558-containing compartment is distinct from endosomes or biosynthetic organelles. Streptolysin-O-mediated guanosine 5′-3-O-(thio)triphosphate loading of Ra2 microglia caused exocytosis of a major complement of cyt b 558 under conditions where lysosomes or endosomes were not mobilized. We establish phagocytic particles and soluble mediators ATP,TNFα, and CD40L as physiological inducers of cyt b 558 exocytosis to the cell surface, and by shRNA knockdown, we identify Rab27A/B as positive or negative regulators of vesicular mobilization to the phagosome or the cell surface, respectively. Exocytosis was followed by clathrin-dependent internalization of cyt b 558, which could be blocked by a dominant negative mutant of the clathrin-coated pit-associated protein Eps15. Re-internalized cyt b 558 did not reach lysosomes but associated with recycling endosomes and undefined vesicular elements. In conclusion, cyt b 558depends on clathrin for internalization, and in activated macrophages NADPH oxidase occupies a Rab27A/B-regulated secretory compartment, which allows rapid agonist-induced redistribution of superoxide production in the cell.

KW - Adenosine Triphosphate

KW - Animals

KW - CD40 Ligand

KW - Calcium-Binding Proteins

KW - Cells, Cultured

KW - Clathrin

KW - Clathrin-Coated Vesicles

KW - Cytochrome b Group

KW - Endosomes

KW - Exocytosis

KW - Intracellular Signaling Peptides and Proteins

KW - Macrophage Activation

KW - Macrophages

KW - Membrane Glycoproteins

KW - Microglia

KW - NADPH Oxidase

KW - Rats

KW - Superoxides

KW - Tumor Necrosis Factor-alpha

KW - rab GTP-Binding Proteins

U2 - 10.1074/jbc.M111.293696

DO - 10.1074/jbc.M111.293696

M3 - Journal article

C2 - 22157766

SN - 0021-9258

VL - 287

SP - 4835

EP - 4852

JO - Journal of Biological Chemistry

JF - Journal of Biological Chemistry

IS - 7

ER -

NADPH oxidase is internalized by clathrin-coated pits and localizes to a Rab27A/B GTPase-regulated secretory compartment in activated macrophages

Abstract

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