98 research outputs found
Josephson tunnel junctions with strong ferromagnetic interlayer
The dependence of the critical current density j_c on the ferromagnetic
interlayer thickness d_F was determined for Nb/Al_2O_3/Cu/Ni/Nb Josephson
tunnel junctions with ferromagnetic \Ni interlayer from very thin film
thicknesses (\sim 1 nm) upwards and classified into F-layer thickness regimes
showing a dead magnetic layer, exchange, exchange + anisotropy and total
suppression of j_c. The Josephson coupling changes from 0 to pi as function of
d_F, and -very close to the crossover thickness- as function of temperature.
The strong suppression of the supercurrent in comparison to non-magnetic
\Nb/Al_2O_3/Cu/Nb junctions indicated that the insertion of a F-layer leads to
additional interface scattering. The transport inside the dead magnetic layer
was in dirty limit. For the magnetically active regime fitting with both the
clean and the dirty limit theory were carried out, indicating dirty limit
condition, too. The results were discussed in the framework of literatureComment: 8 pages, 5 pictures v2: major conceptual change
Josephson tunnel junctions with ferromagnetic \Fe_{0.75}\Co_{0.25} barriers
Josephson tunnel junctions with the strong ferromagnetic alloy
\Fe_{0.75}\Co_{0.25} as the barrier material were studied. The junctions were
prepared with high quality down to a thickness range of a few monolayers of
Fe-Co. An oscillation length of between 0
and -Josephson phase coupling and a very short decay length
for the amplitude of the superconducting
pair wave function in the Fe-Co layer were determined. The rapid damping of the
pair wave function inside the Fe-Co layer is caused by the strong ferromagnetic
exchange field and additional magnetic pair breaking scattering. Josephson
junctions with Fe-Co barriers show a significantly increased tendency towards
magnetic remanence and flux trapping for larger thicknesses .Comment: contains 5 figure
STUDY OF MODIFIED HEAT-SHIELDING COATINGS BASED ON ZrO2
The methods for modifying heat-shielding coatings by applying a layer based on ZrO2 followed by drying and calcination at 1200Β°C in an inert atmosphere have been developed
Multibudded tubules formed by COPII on artificial liposomes
COPII-coated vesicles form at the endoplasmic reticulum for cargo transport to the Golgi apparatus. We used in vitro reconstitution to examine the roles of the COPII scaffold in remodeling the shape of a lipid bilayer. Giant Unilamellar Vesicles were examined using fast confocal fluorescence and cryo-electron microscopy in order to avoid separation steps and minimize mechanical manipulation. COPII showed a preference for high curvature structures, but also sufficient flexibility for binding to low curvatures. The COPII proteins induced beads-on-a-string-like constricted tubules, similar to those previously observed in cells. We speculate about a mechanical pathway for vesicle fission from these multibudded COPII-coated tubules, considering the possibility that withdrawal of the Sar1 amphipathic helix upon GTP hydrolysis leads to lipid bilayer destabilization resulting in fission
Loss of PTEN Is Not Associated with Poor Survival in Newly Diagnosed Glioblastoma Patients of the Temozolomide Era
Introduction: Pre-temozolomide studies demonstrated that loss of the tumor suppressor gene PTEN held independent prognostic significance in GBM patients. We investigated whether loss of PTEN predicted shorter survival in the temozolomide era. The role of PTEN in the PI3K/Akt pathway is also reviewed. Methods: Patients with histologically proven newly diagnosed GBM were identified from a retrospective database between 2007 and 2010. Cox proportional hazards analysis was used to calculate the independent effects of PTEN expression, age
ADP Ribosylation Factors 1 and 4 and Group VIA Phospholipase A2 Regulate Morphology and Intraorganellar Traffic in the Endoplasmic ReticulumβGolgi Intermediate Compartment
In search of morphological determinants for the endoplasmic reticulum-Golgi intermediate compartment (ERGIC), we found that a concerted action of Arf1, Arf4, and PLA2G6-A controls the architecture of the ERGIC by regulating tubular carriers. This is predicted to impact the rate of transport and destination of cargos in the ERGIC
Topology of molecular machines of the endoplasmic reticulum: a compilation of proteomics and cytological data
The endoplasmic reticulum (ER) is a key organelle of the secretion pathway involved in the synthesis of both proteins and lipids destined for multiple sites within and without the cell. The ER functions to both co- and post-translationally modify newly synthesized proteins and lipids and sort them for housekeeping within the ER and for transport to their sites of function away from the ER. In addition, the ER is involved in the metabolism and degradation of specific xenobiotics and endogenous biosynthetic products. A variety of proteomics studies have been reported on different subcompartments of the ER providing an ER protein dictionary with new data being made available on many protein complexes of relevance to the biology of the ER including the ribosome, the translocon, coatomer proteins, cytoskeletal proteins, folding proteins, the antigen-processing machinery, signaling proteins and proteins involved in membrane traffic. This review examines proteomics and cytological data in support of the presence of specific molecular machines at specific sites or subcompartments of the ER
The Biochemistry, Ultrastructure, and Subunit Assembly Mechanism of AMPA Receptors
The AMPA-type ionotropic glutamate receptors (AMPA-Rs) are tetrameric ligand-gated ion channels that play crucial roles in synaptic transmission and plasticity. Our knowledge about the ultrastructure and subunit assembly mechanisms of intact AMPA-Rs was very limited. However, the new studies using single particle EM and X-ray crystallography are revealing important insights. For example, the tetrameric crystal structure of the GluA2cryst construct provided the atomic view of the intact receptor. In addition, the single particle EM structures of the subunit assembly intermediates revealed the conformational requirement for the dimer-to-tetramer transition during the maturation of AMPA-Rs. These new data in the field provide new models and interpretations. In the brain, the native AMPA-R complexes contain auxiliary subunits that influence subunit assembly, gating, and trafficking of the AMPA-Rs. Understanding the mechanisms of the auxiliary subunits will become increasingly important to precisely describe the function of AMPA-Rs in the brain. The AMPA-R proteomics studies continuously reveal a previously unexpected degree of molecular heterogeneity of the complex. Because the AMPA-Rs are important drug targets for treating various neurological and psychiatric diseases, it is likely that these new native complexes will require detailed mechanistic analysis in the future. The current ultrastructural data on the receptors and the receptor-expressing stable cell lines that were developed during the course of these studies are useful resources for high throughput drug screening and further drug designing. Moreover, we are getting closer to understanding the precise mechanisms of AMPA-R-mediated synaptic plasticity
Association of Calcineurin with the COPI Protein Sec28 and the COPII Protein Sec13 Revealed by Quantitative Proteomics
Calcineurin is a calcium-calmodulin-dependent serine/threonine specific protein phosphatase operating in key cellular processes governing responses to extracellular cues. Calcineurin is essential for growth at high temperature and virulence of the human fungal pathogen Cryptococcus neoformans but the underlying mechanism is unknown. We performed a mass spectrometry analysis to identify proteins that associate with the calcineurin A catalytic subunit (Cna1) in C. neoformans cells grown under non-stress and high temperature stress conditions. A novel prioritization strategy for mass spectrometry data from immunoprecipitation experiments identified putative substrates and proteins potentially operating with calcineurin in common pathways. Cna1 co-purified with proteins involved in membrane trafficking including the COPI component Sec28 and the COPII component Sec13. The association of Cna1 with Sec28 and Sec13 was confirmed by co-immunoprecipitation. Cna1 exhibited a dramatic change in subcellular localization during high temperature stress from diffuse cytoplasmic to ER-associated puncta and the mother-bud neck and co-localized with Sec28 and Sec13
- β¦