Myosin light chain kinase is not a regulator of synaptic vesicle trafficking during repetitive exocytosis in cultured hippocampal neurons

The mechanism by which synaptic vesicles (SVs) are recruited to the release site is poorly understood. One candidate mechanism for trafficking of SVs is the myosin-actin motor system. Myosin activity is modulated by myosin light chain kinase (MLCK), which in turn is activated by calmodulin. Ca2+ signaling in presynaptic terminals, therefore, may serve to regulate SV mobility along actin filaments via MLCK. Previous studies in different types of synapses have supported such a hypothesis. Here, we further investigated the role of MLCK in neurotransmitter release at glutamatergic synapses in cultured hippocampal neurons by examining the effects of two MLCK inhibitors, 1-(5-iodonaphthalene-1-sulfonyl)-1H-hexahydro-1,4-diazepine(.)HCl (ML-7) and wortmannin. Bath application of ML-7 enhanced short-term depression of EPSCs to repetitive stimulation, whereas it reduced presynaptic release probability. However, ML-7 also inhibited action potential amplitude and voltage-gated Ca2+ channel currents. These effects were not mimicked by wortmannin, suggesting that ML-7 was not specific to MLCK in hippocampal neurons. When SV exocytosis was directly triggered by a Ca2+ ionophore, calcimycin, to bypass voltage-gated Ca2+ channels, ML-7 had no effect on neurotransmitter release. Furthermore, when SV exocytosis elicited by electrical field stimulation was monitored by styryl dye, FM1-43 [N-(3-triethylammoniumpropyl)-4-(4-( dibutylamino) styryl) pyridinium dibromide], the unloading kinetics of the dye was not altered in the presence of wortmannin. These data indicate that MLCK is not a major regulator of presynaptic SV trafficking during repetitive exocytosis at hippocampal synapses

Magnetic record support

The magnetic layer of a magnetic record support is coated with a thin film of a polymer with a siloxane bond. The magnetic layer consists of a thin film obtained by vacuum metallization, cathode sputtering or dispersion of a ferromagnetic metal powder in a binder. The polymer with a siloxane bond is produced by the polymerization of an organic silicon compound which inherently contains or is able to form this bond. Polymerization is preferably performed by plasma polymerization

Shimanto geosyncline and Kuroshio paleoland

The late Mesozoic to early Neogene geosyncline in the Outer zone of Southwest Japan has been studied in detail in the Kii Peninsula by the Research Group for the Shimanto Geosyncline. The existence of the Kuroshio Paleoland to the south of the geosyncline was inferred by various sedimentologic evidences. The Shimanto belt in the Kii Peninsula is divided from north to south into three zones of Cretaceous, Eocene and Oligocene to lower Miocene. In these belts thick geosynclinal sediments were accumulated showing coarsening upward. The southward migration of the basin occurred in Cretaceous/Eocene, Eocene/Oligocene, and in early Miocene. In the present paper the reconstruction of paleogeography of the Shimanto geosyncline was attempted and the Kuroshio Paleoland was discussed in relation to the geohistory of the Philippine Sea. In spite of the detailed geologic survey in the Kii Peninsula there is no evidence of large exotic blocks nor tectonic mélanges, and this does not support the plate tectonic model ofthe Pacific-type orogeny for the Shimanto belt.ArticleJournal of Physics of the Earth. 26(suppl):357-366 (1978)journal articl

Draft Genome Sequencing and Comparative Analysis of Aspergillus sojae NBRC4239

We conducted genome sequencing of the filamentous fungus Aspergillus sojae NBRC4239 isolated from the koji used to prepare Japanese soy sauce. We used the 454 pyrosequencing technology and investigated the genome with respect to enzymes and secondary metabolites in comparison with other Aspergilli sequenced. Assembly of 454 reads generated a non-redundant sequence of 39.5-Mb possessing 13 033 putative genes and 65 scaffolds composed of 557 contigs. Of the 2847 open reading frames with Pfam domain scores of >150 found in A. sojae NBRC4239, 81.7% had a high degree of similarity with the genes of A. oryzae. Comparative analysis identified serine carboxypeptidase and aspartic protease genes unique to A. sojae NBRC4239. While A. oryzae possessed three copies of α-amyalse gene, A. sojae NBRC4239 possessed only a single copy. Comparison of 56 gene clusters for secondary metabolites between A. sojae NBRC4239 and A. oryzae revealed that 24 clusters were conserved, whereas 32 clusters differed between them that included a deletion of 18 508 bp containing mfs1, mao1, dmaT, and pks-nrps for the cyclopiazonic acid (CPA) biosynthesis, explaining the no productivity of CPA in A. sojae. The A. sojae NBRC4239 genome data will be useful to characterize functional features of the koji moulds used in Japanese industries

Cdk5 Is Involved in BDNF-Stimulated Dendritic Growth in Hippocampal Neurons

Neurotrophins are key regulators of neuronal survival and differentiation during development. Activation of their cognate receptors, Trk receptors, a family of receptor tyrosine kinases (RTKs), is pivotal for mediating the downstream functions of neurotrophins. Recent studies reveal that cyclin-dependent kinase 5 (Cdk5), a serine/threonine kinase, may modulate RTK signaling through phosphorylation of the receptor. Given the abundant expression of both Cdk5 and Trk receptors in the nervous system, and their mutual involvement in the regulation of neuronal architecture and synaptic functions, it is of interest to investigate if Cdk5 may also modulate Trk signaling. In the current study, we report the identification of TrkB as a Cdk5 substrate. Cdk5 phosphorylates TrkB at Ser478 at the intracellular juxtamembrane region of TrkB. Interestingly, attenuation of Cdk5 activity or overexpression of a TrkB mutant lacking the Cdk5 phosphorylation site essentially abolishes brain-derived neurotrophic factor (BDNF)–triggered dendritic growth in primary hippocampal neurons. In addition, we found that Cdk5 is involved in BDNF-induced activation of Rho GTPase Cdc42, which is essential for BDNF-triggered dendritic growth. Our observations therefore reveal an unanticipated role of Cdk5 in TrkB-mediated regulation of dendritic growth through modulation of BDNF-induced Cdc42 activation

Updated Measurements of [O iii] 88 μm, [C ii] 158 μm, and Dust Continuum Emission from a z = 7.2 Galaxy

We present updated measurements of the [O iii] 88 μm, [C ii] 158 μm, and dust continuum emission from a star-forming galaxy at z = 7.212, SXDF-NB1006-2, by utilizing Atacama Large Millimeter/submillimeter Array (ALMA) archival data sets analysed in previous studies and data sets that have not been analysed before. The follow-up ALMA observations with higher angular resolution and sensitivity reveal a clumpy structure of the [O iii] emission on a scale of 0.32-0.85 kpc. We also combined all the ALMA [O iii] ([C ii]) data sets and updated the [O iii] ([C ii]) detection to 5.9σ (3.6σ-4.5σ). The non-detection of [C ii] with data from the REBELS large program implies the incompleteness of spectral-scan surveys using [C ii] to detect galaxies with high star formation rates (SFRs) but marginal [C ii] emission at high-z. The dust continuum at 90 and 160 μm remains undetected, indicating little dust content of <3.9 × 106 M ⊙ (3σ), and we obtained a more stringent constraint on the total infrared luminosity. We updated the [O iii]/[C ii] luminosity ratios to 10.2 ± 4.7 (6.1 ± 3.5) and 20 ± 12 (9.6 ± 6.1) for the 4.5σ and 3.6σ [C ii] detections, respectively, where the ratios in the parentheses are corrected for the surface brightness dimming effect on the extended [C ii] emission. We also found a strong [C ii] deficit (0.6-1.3 dex) between SXDF-NB1006-2 and the mean L [C II]−SFR relation of galaxies at 0 < z < 9

Presynaptically Localized Cyclic GMP-Dependent Protein Kinase 1 Is a Key Determinant of Spinal Synaptic Potentiation and Pain Hypersensitivity

Electrophysiological and behavioral experiments in mice reveal that a cGMP-dependent kinase amplifies neurotransmitter release from peripheral pain sensors, potentiates spinal synapses, and leads to exaggerated pain

Platelet Activating Factor Blocks Interkinetic Nuclear Migration in Retinal Progenitors through an Arrest of the Cell Cycle at the S/G2 Transition

Nuclear migration is regulated by the LIS1 protein, which is the regulatory subunit of platelet activating factor (PAF) acetyl-hydrolase, an enzyme complex that inactivates the lipid mediator PAF. Among other functions, PAF modulates cell proliferation, but its effects upon mechanisms of the cell cycle are unknown. Here we show that PAF inhibited interkinetic nuclear migration (IKNM) in retinal proliferating progenitors. The lipid did not, however, affect the velocity of nuclear migration in cells that escaped IKNM blockade. The effect depended on the PAF receptor, Erk and p38 pathways and Chk1. PAF induced no cell death, nor a reduction in nucleotide incorporation, which rules out an intra-S checkpoint. Notwithstanding, the expected increase in cyclin B1 content during G2-phase was prevented in the proliferating cells. We conclude that PAF blocks interkinetic nuclear migration in retinal progenitor cells through an unusual arrest of the cell cycle at the transition from S to G2 phases. These data suggest the operation, in the developing retina, of a checkpoint that monitors the transition from S to G2 phases of the cell cycle