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izvor podataka: crosbi

GFP-golvesin constructs to study Golgi tubulation and post-Golgi vesicle dynamics in phagocytosis (CROSBI ID 106080)

Prilog u časopisu | izvorni znanstveni rad | međunarodna recenzija

Gerisch, G. ; Benjak, A. ; Köhler, J. ; Weber, Igor ; Schneider, N. GFP-golvesin constructs to study Golgi tubulation and post-Golgi vesicle dynamics in phagocytosis // European journal of cell biology, 83 (2004), 297-303-x

Podaci o odgovornosti

Gerisch, G. ; Benjak, A. ; Köhler, J. ; Weber, Igor ; Schneider, N.

engleski

GFP-golvesin constructs to study Golgi tubulation and post-Golgi vesicle dynamics in phagocytosis

Dictyostelium cells are professional phagocytes that are optimally suited for the imaging of phagosome processing from particle uptake to exocytosis. In order to design fluorescent probes for monitoring membrane trafficking in the endocytic pathway, we have dissected a membrane protein, golvesin, and have linked fragments of its sequence to GFP. Endogenous golvesin is partitioned between the ER, the Golgi apparatus, endosomes, and the contractile vacuole complex. We have localized signals that are required for exit from the Golgi to post-Golgi compartments to the C-terminal region of the golvesin sequence. One GFP-tagged fragment turned out to be a highly specific Golgi marker and was used to demonstrate the interaction of Golgi tubules with phagosomes. Signals essential for the retrieval of golvesin at the end of phagosome processing were localized to the N-terminal region. A truncated golvesin construct escaping retrieval was employed in recording the delivery of a phagosomal protein to the plasma membrane. During exocytosis of a phagosome filled with multiple particles, this construct made a segmentation process visible, meaning that membrane fusions alternate with sequential release of the particles.

Exocytosis; Golgi tubules; Membrane fusion; Membrane trafficking; Phagocytosis

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Podaci o izdanju

83

2004.

297-303-x

objavljeno

0171-9335

Povezanost rada

Biologija

Indeksiranost