synaptojanin1 Is Required for Temporal Fidelity of Synaptic Transmission in Hair Cells

To faithfully encode mechanosensory information, auditory/vestibular hair cells utilize graded synaptic vesicle (SV) release at specialized ribbon synapses. The molecular basis of SV release and consequent recycling of membrane in hair cells has not been fully explored. Here, we report that comet, a gene identified in an ENU mutagenesis screen for zebrafish larvae with vestibular defects, encodes the lipid phosphatase Synaptojanin 1 (Synj1). Examination of mutant synj1 hair cells revealed basal blebbing near ribbons that was dependent on Cav1.3 calcium channel activity but not mechanotransduction. Synaptojanin has been previously implicated in SV recycling; therefore, we tested synaptic transmission at hair-cell synapses. Recordings of post-synaptic activity in synj1 mutants showed relatively normal spike rates when hair cells were mechanically stimulated for a short period of time at 20 Hz. In contrast, a sharp decline in the rate of firing occurred during prolonged stimulation at 20 Hz or stimulation at a higher frequency of 60 Hz. The decline in spike rate suggested that fewer vesicles were available for release. Consistent with this result, we observed that stimulated mutant hair cells had decreased numbers of tethered and reserve-pool vesicles in comparison to wild-type hair cells. Furthermore, stimulation at 60 Hz impaired phase locking of the postsynaptic activity to the mechanical stimulus. Following prolonged stimulation at 60 Hz, we also found that mutant synj1 hair cells displayed a striking delay in the recovery of spontaneous activity. Collectively, the data suggest that Synj1 is critical for retrieval of membrane in order to maintain the quantity, timing of fusion, and spontaneous release properties of SVs at hair-cell ribbon synapses.     

Golgi- and Trans-Golgi Network-Mediated Vesicle Trafficking Is Required for Wax Secretion from Epidermal Cells

Lipid secretion from epidermal cells to the plant surface is essential to create the protective plant cuticle. Cuticular waxes are unusual secretory products, consisting of a variety of highly hydrophobic compounds including saturated very-long-chain alkanes, ketones, and alcohols. These compounds are synthesized in the endoplasmic reticulum (ER) but must be trafficked to the plasma membrane for export by ATP-binding cassette transporters. To test the hypothesis that wax components are trafficked via the endomembrane system and packaged in Golgi-derived secretory vesicles, Arabidopsis (Arabidopsis thaliana) stem wax secretion was assayed in a series of vesicle-trafficking mutants, including gnom like1-1 (gnl1-1), transport particle protein subunit120-4, and echidna (ech). Wax secretion was dependent upon GNL1 and ECH. Independent of secretion phenotypes, mutants with altered ER morphology also had decreased wax biosynthesis phenotypes, implying that the biosynthetic capacity of the ER is closely related to its structure. These results provide genetic evidence that wax export requires GNL1- and ECH-dependent endomembrane vesicle trafficking to deliver cargo to plasma membrane-localized ATP-binding cassette transporters.The aerial, nonwoody tissues of all land plants are covered by a waxy cuticle that protects the plant against nonstomatal water loss. The cuticle also provides the first barrier between the plant and its environment and mediates important biotic and abiotic interactions. The cuticle has two main components: cutin and waxes. Cutin is a tough, cross-linked polyester matrix primarily composed of C16 and C18 oxygenated fatty acids and glycerol (Pollard et al., 2008). Wax is a heterogenous mixture, primarily composed of very-long-chain (VLC) fatty acid derivatives (predominantly 29-carbon alkane in Arabidopsis [Arabidopsis thaliana] stems).As a result of biochemical approaches, forward genetic screens yielding the eceriferum (cer) mutants (Koornneef et al., 1989), and reverse genetics approaches (Greer et al., 2007), almost all of the enzymes in the wax biosynthesis pathway have been identified. The enzymes that elongate C16 or C18 fatty acids to VLC (greater than 20C) fatty acids are localized in the endoplasmic reticulum (ER; for review, see Haslam and Kunst, 2013). Primary alcohols are synthesized by the fatty acyl reductases (Rowland et al., 2006), while alkanes are generated via an undefined mechanism involving CER1, CER3, and an unidentified cytochrome b₅ (Bernard et al., 2012). These alkanes may be modified by the midchain alkane hydroxylase cytochrome P450 (MAH1) to generate secondary alcohols and ketones (Greer et al., 2007). All of these wax synthesis enzymes have also been localized to the ER (Greer et al., 2007; Bernard et al., 2012).In contrast to wax synthesis, comparatively little is known about how waxes are trafficked within the cell from their site of synthesis at the ER to the plasma membrane. ATP-binding cassette (ABC) transporters of the G subfamily are required for wax export, and when either half-transporter is disrupted, waxes accumulate in the ER (McFarlane et al., 2010). Two extracellular glycosylphosphatidylinositol-anchored lipid transfer proteins (LTPs) are further required for wax accumulation on the plant surface (DeBono et al., 2009; Kim et al., 2012). Although these components of the molecular machinery of wax transport at the plasma membrane have been identified, the intracellular mechanisms by which waxes are transported to the plasma membrane remain undefined.Several mechanisms have been hypothesized for the transport of waxes from the ER to the plasma membrane (for review, see Samuels et al., 2008). Waxes could be incorporated into vesicles at the ER, travel to and through the Golgi apparatus and the trans-Golgi network (TGN), and then move to the plasma membrane via vesicle secretion. These vesicles could carry wax components within their membranes, as computational modeling of wax components in lipid bilayers indicates that VLC alkanes partition entirely into the hydrophobic phase of the bilayer (Coll et al., 2007). Alternatively, lipoproteins may bind to lipid molecules in order to solubilize them so that they can be transported as cargo in the vesicle lumen, by analogy to mammalian systems where lipoproteins are secreted from hepatocytes into the circulatory system by exocytosis via post-Golgi vesicles (for review, see Mansbach and Siddiqi, 2010). However, no analogous lipid-binding apoproteins or transport vesicles have been found in plants. It is also possible that LTPs in membrane contact sites between the ER and the plasma membrane could transfer cuticular lipids directly from the ER to the plasma membrane. However, although these membrane contact sites have been observed in plant cells (Samuels and McFarlane, 2012), no structural or functional components of membrane contact sites are known.Early studies of VLC fatty acid trafficking used pulse-chase labeling to show that treatment with monensin, a post-Golgi trafficking inhibitor, results in decreased VLC fatty acid trafficking to the plasma membrane and a corresponding increase in these lipids in the Golgi apparatus (Bertho et al., 1991), suggesting a Golgi-dependent mechanism of VLC lipid trafficking to the plasma membrane. However, the “Golgi” fraction in this study contained significant elongase activity, which has subsequently been localized to the ER, making interpretation of these data difficult. While a variety of inhibitors are available that disrupt different stages in the secretory pathway (Zhang et al., 1993; Robinson et al., 2008), inhibitor studies of wax trafficking have proven ineffective, since the wax-producing epidermal cells do not effectively take up solutions carrying these inhibitors. This illustrates the difficulties of studying the transport of highly hydrophobic cargo, such as wax, within the single cell layer of epidermis.The objective of this study was to determine the intracellular trafficking mechanisms underlying cuticular wax transport from the ER to the plasma membrane. Arabidopsis mutants, which have been successfully applied in wax biosynthesis studies, were used to investigate wax secretion. Well-characterized mutants with defects in vesicle traffic and protein secretion were chosen to test the hypothesis that wax components are trafficked via endomembrane vesicles. These mutant analyses indicate that wax movement from the ER to the plasma membrane requires vesicle traffic at both the ER-Golgi interface and the TGN. Independent of secretion phenotypes, strong decreases in wax synthesis were observed in mutants with altered ER morphology, which implies that ER structure influences its biosynthetic capacity for wax production.     

Synaptotagmin IV Modulation of Vesicle Size and Fusion Pores in PC12 Cells

Many synaptotagmins are Ca²⁺-binding membrane proteins with functions in Ca²⁺-triggered exocytosis. Synaptotagmin IV (syt IV) has no Ca²⁺ binding activity, but nevertheless modulates exocytosis. Here, cell-attached capacitance recording was used to study single vesicle fusion and fission in control and syt IV overexpressing PC12 cells. Unitary capacitance steps varied widely in size, indicating that both microvesicles (MVs) and dense-core vesicles (DCVs) undergo fusion. Syt IV overexpression reduced the size of DCVs and endocytotic vesicles but not MVs. Syt IV also reduced the basal rate of Ca²⁺-induced fusion. During kiss-and-run, syt IV increased the conductance and duration of DCV fusion pores but not MV fusion pores. During full-fusion of DCVs syt IV increased the fusion pore conductance but not the duration. Syt IV overexpression increased the duration but not the conductance of fission pores during endocytosis. The effects of syt IV on fusion pores in PC12 cells resembled the effects on fusion pores in peptidergic nerve terminals. However, differences between these and results obtained with amperometry may indicate that amperometry and capacitance detect the fusion of different populations of vesicles. The effects of syt IV on fusion pores are discussed in terms of structural models and kinetic mechanisms.     

Immunocytochemical Localization of Synaptic Proteins at Vesicular Organelles in PC12 Cells

The distribution of the three synaptic vesicle proteins SV2, synaptophysin and synaptotagmin, and of SNAP-25, a component of the docking and fusion complex, was investigated in PC12 cells by immunocytochemistry. Colloidal gold particle-bound secondary antibodies and a preembedding protocol were applied. Granules were labeled for SV2 and synaptotagmin but not for synaptophysin. Electron-lucent vesicles were labeled most intensively for synaptophysin but also for SV2 and to a lesser extent for synaptotagmin. The t-SNARE SNAP-25 was found at the plasma membrane but also at the surface of granules. Labeling of Golgi vesicles was observed for all antigens investigated. Also components of the endosomal pathway such as multivesicular bodies and multilamellar bodies were occasionally marked. The results suggest that the three membrane-integral synaptic vesicle proteins can have a differential distribution between electron-lucent vesicles (of which PC12 cells may possess more than one type) and granules. The membrane compartment of granules appears not to be an immediate precursor of that of electron-lucent vesicles.     

Mdm12p, a Component Required for Mitochondrial Inheritance That Is Conserved between Budding and Fission Yeast

Saccharomyces cerevisiae cells lacking the MDM12 gene product display temperature-sensitive growth and possess abnormally large, round mitochondria that are defective for inheritance by daughter buds. Analysis of the wild-type MDM12 gene revealed its product to be a 31-kD polypeptide that is homologous to a protein of the fission yeast Schizosaccharomyces pombe. When expressed in S. cerevisiae, the S. pombe Mdm12p homolog conferred a dominant-negative phenotype of giant mitochondria and aberrant mitochondrial distribution, suggesting partial functional conservation of Mdm12p activity between budding and fission yeast. The S. cerevisiae Mdm12p was localized by indirect immunofluorescence microscopy and by subcellular fractionation and immunodetection to the mitochondrial outer membrane and displayed biochemical properties of an integral membrane protein. Mdm12p is the third mitochondrial outer membrane protein required for normal mitochondrial morphology and distribution to be identified in S. cerevisiae and the first such mitochondrial component that is conserved between two different species.     

Synaptojanin 1 Is Required for Endolysosomal Trafficking of Synaptic Proteins in Cone Photoreceptor Inner Segments

Highly polarized cells such as photoreceptors require precise and efficient strategies for establishing and maintaining the proper subcellular distribution of proteins. The signals and molecular machinery that regulate trafficking and sorting of synaptic proteins within cone inner segments is mostly unknown. In this study, we show that the polyphosphoinositide phosphatase Synaptojanin 1 (SynJ1) is critical for this process. We used transgenic markers for trafficking pathways, electron microscopy, and immunocytochemistry to characterize trafficking defects in cones of the zebrafish mutant, nrc^a14, which is deficient in phosphoinositide phosphatase, SynJ1. The outer segments and connecting cilia of nrc^a14 cone photoreceptors are normal, but RibeyeB and VAMP2/synaptobrevin, which normally localize to the synapse, accumulate in the nrc^a14 inner segment. The structure of the Endoplasmic Reticulum in nrc^a14 mutant cones is normal. Golgi develop normally, but later become disordered. Large vesicular structures accumulate within nrc^a14 cone photoreceptor inner segments, particularly after prolonged incubation in darkness. Cone inner segments of nrc ^a14 mutants also have enlarged acidic vesicles, abnormal late endosomes, and a disruption in autophagy. This last pathway also appears exacerbated by darkness. Taken altogether, these findings show that SynJ1 is required in cones for normal endolysosomal trafficking of synaptic proteins.     

Rab3D Is Critical for Secretory Granule Maturation in PC12 Cells

Neuropeptide- and hormone-containing secretory granules (SGs) are synthesized at the trans-Golgi network (TGN) as immature secretory granules (ISGs) and complete their maturation in the F-actin-rich cell cortex. This maturation process is characterized by acidification-dependent processing of cargo proteins, condensation of the SG matrix and removal of membrane and proteins not destined to mature secretory granules (MSGs). Here we addressed a potential role of Rab3 isoforms in these maturation steps by expressing their nucleotide-binding deficient mutants in PC12 cells. Our data show that the presence of Rab3D(N135I) decreases the restriction of maturing SGs to the F-actin-rich cell cortex, blocks the removal of the endoprotease furin from SGs and impedes the processing of the luminal SG protein secretogranin II. This strongly suggests that Rab3D is implicated in the subcellular localization and maturation of ISGs.     

Dopamine-Induced Apoptosis Is Inhibited in PC12 Cells Expressing Bcl-2

1. Degeneration of nigrostriatal dopaminergic neurons is the major pathogenic substrate of Parkinson's disease (PD). It is assumed that the lethal trigger is the accumulation of oxidative reactive species generated during metabolism of the natural neurotransmitter dopamine.2. We have recently shown that dopamine is capable of inducing programmed cell death (PCD) or apoptosis in cultured postmitotic chick sympathetic neurons and rat PC12 pheochromocytoma cells.3. The bcl-2 gene encodes a protein which blocks physiological PCD in many mammalian cells. In an attempt to elucidate further the mechanism of dopamine toxicity, we examined the potential protective effect of bcl-2 in PC12 cells which were transfected with the protooncogene.4. In our experiments, Bcl-2 producing cells showed a marked resistance to dopamine toxicity. The percentage of nuclear condensation and DNA fragmentation visualized by the end-labeling method following dopamine treatment was significantly lower in bcl-2 expressing cells. Bcl-2 did not protect PC12 cells against toxicity induced by exposure to dopamine-melanin. Extracts of PC12 cells containing Bcl-2 inhibited dopamine autooxidation and formation of dopamine-melanin. Furthermore, the presence of Bcl-2 protected cells from thiol imbalance and prevented thiol loss following exposure to dopamine.5. The protective effects of Bcl-2 against dopamine toxicity may be explained, in part, by its action as an antioxidant and by its interference in the production of toxic agents. The possible protection by Bcl-2 against neuronal degeneration caused by dopamine may play a role in the pathogenesis of PD andmay provide a new direction for the development of neuroprotective therapies.     

Nucleolar Integrity Is Required for the Maintenance of Long-Term Synaptic Plasticity

Long-term memory (LTM) formation requires new protein synthesis and new gene expression. Based on our work in Aplysia, we hypothesized that the rRNA genes, stimulation-dependent targets of the enzyme Poly(ADP-ribose) polymerase-1 (PARP-1), are primary effectors of the activity-dependent changes in synaptic function that maintain synaptic plasticity and memory. Using electrophysiology, immunohistochemistry, pharmacology and molecular biology techniques, we show here, for the first time, that the maintenance of forskolin-induced late-phase long-term potentiation (L-LTP) in mouse hippocampal slices requires nucleolar integrity and the expression of new rRNAs. The activity-dependent upregulation of rRNA, as well as L-LTP expression, are poly(ADP-ribosyl)ation (PAR) dependent and accompanied by an increase in nuclear PARP-1 and Poly(ADP) ribose molecules (pADPr) after forskolin stimulation. The upregulation of PARP-1 and pADPr is regulated by Protein kinase A (PKA) and extracellular signal-regulated kinase (ERK)—two kinases strongly associated with long-term plasticity and learning and memory. Selective inhibition of RNA Polymerase I (Pol I), responsible for the synthesis of precursor rRNA, results in the segmentation of nucleoli, the exclusion of PARP-1 from functional nucleolar compartments and disrupted L-LTP maintenance. Taken as a whole, these results suggest that new rRNAs (28S, 18S, and 5.8S ribosomal components)—hence, new ribosomes and nucleoli integrity—are required for the maintenance of long-term synaptic plasticity. This provides a mechanistic link between stimulation-dependent gene expression and the new protein synthesis known to be required for memory consolidation.     

Multiple Levels for Regulation of TrkA in PC12 Cells by Nerve Growth Factor

Abstract: TrkA is a receptor tyrosine kinase for nerve growth factor (NGF). Recent studies indicate that NGF regulates not only activation of trkA kinase but also expression of the trkA gene. To further define NGF actions on trkA, we examined binding and signaling through trkA after both short and long intervals of NGF treatment. Induction of tyrosine phosphorylation on gp140 ^trkA was rapidly followed by down-regulation of cell surface and total cellular gp140 ^trkA . At later intervals, increased expression of trkA was evident in increased mRNA and protein levels. At 7 days, there was increased binding to gp140 ^trkA and increased signaling through this receptor. NGF appears to regulate trkA at several levels. In neurons persistently exposed to NGF, maintenance of NGF signaling may require increased trkA gene expression.     

ADP Ribosylation Factor Like 2 (Arl2) Regulates Breast Tumor Aggressivity in Immunodeficient Mice

We have previously reported that ADP ribosylation factor like 2 (Arl2), a small GTPase, content influences microtubule dynamics and cell cycle distribution in breast tumor cells, as well as the degree and distribution of phosphorylated P53. Here we show, in two different human breast adenocarcinoma models, that Arl2 content has a major impact on breast tumor cell aggressivity both in vitro and in vivo. Cells with reduced content of Arl2 displayed reduced contact inhibition, increased clonogenic or cluster formation as well as a proliferative advantage over control cells in an in vitro competition assay. These cells also caused larger tumors in SCID mice, a phenotype which was mimicked by the in vivo administration of siRNA directed against Arl2. Cells with increased Arl2 content displayed reduced aggressivity, both in vitro and in vivo, with enhanced necrosis and were also found to contain increased PP2A phosphatase activity. A rt-PCR analysis of fresh human tumor breast samples suggested that low Arl2 expression was associated with larger tumor size and greater risk of lymph node involvement at diagnosis. These data underline the role of Arl2, a small GTPase, as an important regulator of breast tumor cell aggressivity, both in vitro and in vivo.