We have recently described a system that recreates in vitro the generation of post-Golgi vesicles from purified Golgi fractions obtained from virus-infected MDCK cells in which the vesicular stomatitis virus-G envelope glycoprotein had been allowed to accumulate in vivo in the TGN. Vesicle formation, monitored by the release of the viral glycoprotein, was shown to require the activation of a GTP-binding ADP ribosylation factor (ARF) protein that promotes the assembly of a vesicle coat in the TGN, and to be regulated by a Golgi-associated protein kinase C (PKC)-like activity. We have now been able to dissect the process of post-Golgi vesicle generation into two sequential stages, one of coat assembly and bud formation, and another of vesicle scission, neither of which requires an ATP supply. The first stage can occur at 20 degrees C, and includes the GTP-dependent activation of the ARF protein, which can be effected by the nonhydrolyzable nucleotide analogue GTP gamma S, whereas the second stage is nucleotide independent and can only occur at a higher temperature of incubation. Cytosolic proteins are required for the vesicle scission step and they cannot be replaced by palmitoyl CoA, which is known to promote, by itself, scission of the coatomer-coated vesicles that mediate intra-Golgi transport. We have found that PKC inhibitors prevented vesicle generation, even when this was sustained by GTP gamma S and ATP levels reduced far below the K(m) of PKC. The inhibitors suppressed vesicle scission without preventing coat assembly, yet to exert their effect, they had to be added before coat assembly took place. This indicates that a target of the putative PKC is activated during the bud assembly stage of vesicle formation, but only acts during the phase of vesicle release. The behavior of the PKC target during vesicle formation resembles that of phospholipase D (PLD), a Golgi-associated enzyme that has been shown to be activated by PKC, even in the absence of the latter's phosphorylating activity. We therefore propose that during coat assembly, PKC activates a PLD that, during the incubation at 37 degrees C, promotes vesicle scission by remodeling the phospholipid bilayer and severing connections between the vesicles and the donor membrane.
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15 October 1996
Article|
October 15 1996
The production of post-Golgi vesicles requires a protein kinase C-like molecule, but not its phosphorylating activity.
J P Simon,
J P Simon
Department of Cell Biology, New York University School of Medicine, New York 10016, USA.
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I E Ivanov,
I E Ivanov
Department of Cell Biology, New York University School of Medicine, New York 10016, USA.
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M Adesnik,
M Adesnik
Department of Cell Biology, New York University School of Medicine, New York 10016, USA.
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D D Sabatini
D D Sabatini
Department of Cell Biology, New York University School of Medicine, New York 10016, USA.
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J P Simon
Department of Cell Biology, New York University School of Medicine, New York 10016, USA.
I E Ivanov
Department of Cell Biology, New York University School of Medicine, New York 10016, USA.
M Adesnik
Department of Cell Biology, New York University School of Medicine, New York 10016, USA.
D D Sabatini
Department of Cell Biology, New York University School of Medicine, New York 10016, USA.
Online ISSN: 1540-8140
Print ISSN: 0021-9525
J Cell Biol (1996) 135 (2): 355–370.
Citation
J P Simon, I E Ivanov, M Adesnik, D D Sabatini; The production of post-Golgi vesicles requires a protein kinase C-like molecule, but not its phosphorylating activity.. J Cell Biol 15 October 1996; 135 (2): 355–370. doi: https://doi.org/10.1083/jcb.135.2.355
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