Phosphatidylinositol-4-Kinase Type II α Is a Component of Adaptor Protein-3-derived Vesicles

Salazar, Gloria; Craige, Branch; Wainer, Bruce H.; Guo, J.; Camilli, Pietro De; Faúndez, Víctor

doi:10.1091/mbc.e05-01-0020

Cited by 99 publications

(160 citation statements)

References 68 publications

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“…We estimate from such data that APP and Mint3 are increased in specific activity Ͼ10-fold over cell homogenate. Although this number may seem low in comparison with a standard protein purification, it is consistent with published procedures for the purification of synaptic (15-18-fold) (Huttner et al, 1983;Floor et al, 1988) or AP-3 (ϳ16-fold; Craige et al, 2005;Salazar et al, 2005) coated vesicles. The fold purification of vesicles was estimated from that of Mint3, which in turn was determined by comparison of immunoreactivity in V6 to serial dilutions of a bacterially expressed recombinant Mint3 standard.…”

supporting

confidence: 87%

“…Magnetic beads (Dynal Biotech, Oslo, Norway), coated with either anti-mouse (M480) or anti-rabbit (M280) immunoglobulin (IgG, were incubated with either mouse monoclonal antibodies to Mint3 or rabbit polyclonal antibody to APP, respectively in PBS/5% bovine serum albumin (BSA) for 2 h at room temperature, according to the Salazar et al (2005). Controls included substitution of either mouse monoclonal or rabbit polyclonal c-myc antibodies.…”

Section: Immunoisolation Of Vesicles and Immunogold Labelingmentioning

confidence: 99%

Section: Enrichment Of App Vesicles From Sh-sy5y Cell Homogenatesmentioning

confidence: 99%

“…Equal amounts of protein from these fractions were then analyzed by immunoblotting to determine where the APP and organelles of the secretory and endocytic membrane traffic fractionated. S2 has been shown previously to contain small vesicles, including synaptic vesicles and coated vesicles, in addition to soluble proteins Salazar et al, 2005), and so was expected to contain a subpopulation of cargos and adaptors that can be used to identify specific vesicles.We found substantial amounts of APP and previously established binding partners, Mints (1-3) and Fe65, in S2 ( Figure 2A). The S2 contained ϳ45-50% of total cell protein under these conditions; yet, it is largely devoid of markers of secretory organelles.…”

mentioning

confidence: 99%

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Mint3/X11γ Is an ADP-Ribosylation Factor-dependent Adaptor that Regulates the Traffic of the Alzheimer's Precursor Protein from theTrans-Golgi Network

Shrivastava-Ranjan

Faúndez

Fang

et al. 2008

MBoC

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␤-Amyloid peptides (A␤) are the major component of plaques in brains of Alzheimer's patients, and are they derived from the proteolytic processing of the ␤-amyloid precursor protein (APP). The movement of APP between organelles is highly regulated, and it is tightly connected to its processing by secretases. We proposed previously that transport of APP within the cell is mediated in part through its sorting into Mint/X11-containing carriers. To test our hypothesis, we purified APP-containing vesicles from human neuroblastoma SH-SY5Y cells, and we showed that Mint2/3 are specifically enriched and that Mint3 and APP are present in the same vesicles. Increasing cellular APP levels increased the amounts of both APP and Mint3 in purified vesicles. Additional evidence supporting an obligate role for Mint3 in traffic of APP from the trans-Golgi network to the plasma membrane include the observations that depletion of Mint3 by small interference RNA (siRNA) or mutation of the Mint binding domain of APP changes the export route of APP from the basolateral to the endosomal/lysosomal sorting route. Finally, we show that increased expression of Mint3 decreased and siRNA-mediated knockdowns increased the secretion of the neurotoxic ␤-amyloid peptide, A␤ 1-40 . Together, our data implicate Mint3 activity as a critical determinant of post-Golgi APP traffic. INTRODUCTIONThe hallmark of Alzheimer's disease is the presence in brain of plaques that contain A␤ peptides, formed by the result of proteolytic processing of the ␤-amyloid precursor protein (APP). APP is a ubiquitous, single-pass transmembrane protein of unknown function that is highly expressed in brain. Processing involves the sequential actions of ␣-or ␤-plus ␥-secretases, each of which are found in multiple cellular locations (Kuentzel et al., 1993;Selkoe, 1998;Yan et al., 2001). Although processing may occur at any step, the trans-Golgi network (TGN) is the earliest site at which APP processing is thought to commence, and APP is internalized from the cell surface to endosomal compartments where ␥-secretase also acts (Selkoe et al., 1996;Greenfield et al., 1999;Lah and Levey, 2000;Bagshaw et al., 2003).The C-terminal domain of APP contains the tyrosinebased sorting motif, YENPTY, which is conserved across species and a determinant of APP traffic (Perez et al., 1999;Bonifacino and Traub, 2003;King et al., 2004). Such sorting motifs function by binding specific adaptors to facilitate their selective import into budding carriers and ensure specificity in cargo selection and coat recruitment. The highly conserved phosphotyrosine binding (PTB) domains in all three Mint proteins have been shown previously to bind directly to the YENPXY motif of APP (Borg et al., 1996(Borg et al., , 1998Zhang et al., 1997;Sastre et al., 1998;Tanahashi and Tabira, 1999;Tomita et al., 1999;Ho et al., 2002;Araki et al., 2003). Other PTB domain containing proteins have similarly been shown to bind APP, including the Fe65 (Sabo et al., 1999) family, Dab2 (Howell et al., 1999), JIP1b (King et al....

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supporting

confidence: 87%

Section: Immunoisolation Of Vesicles and Immunogold Labelingmentioning

confidence: 99%

Section: Enrichment Of App Vesicles From Sh-sy5y Cell Homogenatesmentioning

confidence: 99%

mentioning

confidence: 99%

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Mint3/X11γ Is an ADP-Ribosylation Factor-dependent Adaptor that Regulates the Traffic of the Alzheimer's Precursor Protein from theTrans-Golgi Network

Shrivastava-Ranjan

Faúndez

Fang

et al. 2008

MBoC

Self Cite

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“…At2g40850 encodes a type II PtdIns 4-kinase, which has been previously named PI4Kg1 (Mueller-Roeber and Pical, 2002). While the function of type II PtdIns 4-kinases in plants is unknown, it has been suggested that in animals, they are involved in the regulation of intracellular trafficking (Wang et al, 2003;Salazar et al, 2005). Thus, the mutant phenotype observed for the At2g40850 insertion line might be caused by a malfunction of this essential cellular process.…”

Section: Identification Of Novel Regulators Of Microsporogenesismentioning

confidence: 99%

Global Expression Profiling Applied to the Analysis of Arabidopsis Stamen Development

et al. 2007

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To obtain detailed information about gene expression during stamen development in Arabidopsis (Arabidopsis thaliana), we compared, by microarray analysis, the gene expression profile of wild-type inflorescences to those of the floral mutants apetala3, sporocyteless/nozzle, and male sterile1 (ms1), in which different aspects of stamen formation are disrupted. These experiments led to the identification of groups of genes with predicted expression at early, intermediate, and late stages of stamen development. Validation experiments using in situ hybridization confirmed the predicted expression patterns. Additional experiments aimed at characterizing gene expression specifically during microspore formation. To this end, we compared the gene expression profiles of wild-type flowers of distinct developmental stages to those of the ms1 mutant. Computational analysis of the datasets derived from this experiment led to the identification of genes that are likely involved in the control of key developmental processes during microsporogenesis. We also identified a large number of genes whose expression is prolonged in ms1 mutant flowers compared to the wild type. This result suggests that MS1, which encodes a putative transcriptional regulator, is involved in the stage-specific repression of these genes. Lastly, we applied reverse genetics to characterize several of the genes identified in the microarray experiments and uncovered novel regulators of microsporogenesis, including the transcription factor MYB99 and a putative phosphatidylinositol 4-kinase.

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Lysosome‐Related Organelles: Modifications of the Lysosome Paradigm

Mantegazza

Marks

2016

Lysosomes: Biology, Diseases, and Therapeutics

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Phosphatidylinositol-4-Kinase Type II α Is a Component of Adaptor Protein-3-derived Vesicles

Cited by 99 publications

References 68 publications

Mint3/X11γ Is an ADP-Ribosylation Factor-dependent Adaptor that Regulates the Traffic of the Alzheimer's Precursor Protein from theTrans-Golgi Network

Mint3/X11γ Is an ADP-Ribosylation Factor-dependent Adaptor that Regulates the Traffic of the Alzheimer's Precursor Protein from theTrans-Golgi Network

Global Expression Profiling Applied to the Analysis of Arabidopsis Stamen Development

Lysosome‐Related Organelles: Modifications of the Lysosome Paradigm

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