1,292 research outputs found

    Compact-Size Low-Profile Wideband Circularly Polarized Omnidirectional Patch Antenna With Reconfigurable Polarizations

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    A compact-size low-profile wideband circularly polarized (CP) omnidirectional antenna with reconfigurable polarizations is presented in this communication. This design is based on a low-profile omnidirectional CP antenna which consists of a vertically polarized microstrip patch antenna working in TM01/TM02 modes and sequentially bended slots etched on the ground plane for radiating horizontally polarized electric field. The combined radiation from both the microstrip patch and the slots leads to a CP omnidirectional radiation pattern. The polarization reconfigurability is realized by introducing PIN diodes on the slots. By electronically controlling the states of the PIN diodes, the effective orientation of the slots on ground plane can be changed dynamically and the polarization of antenna can be altered between left-hand circular polarization (LHCP) and right-hand circular polarization (RHCP). The proposed antenna exhibits a wide-operational bandwidth of 19.8% (2.09-2.55 GHz) with both axial ratio below 3 dB and return loss above 10 dB when radiates either LHCP or RHCP waves. Experimental results show good agreement with the simulation results. The present design has a compact size, a thickness of only 0.024? and exhibits stable CP omnidirectional conical-beam radiation patterns within the entire operating frequency band with good circular polarization

    Dimethano­lbis[N′-(3-pyridylmethyl­ene)benzohydrazide]sodium(I) iodide

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    The molecule of the title compound, [Na(C13H11N3O)2(CH3OH)2]I, is non-planar, with the Na atom chelated by the O atoms and the N atoms of two N′-(3-pyridylmethyl­ene)benzohydrazide ligands and both O atoms of two methanol ligands. The asymmetric unit consists of one half-mol­ecule. The Na atom is located on a crystallographic centre of inversion. The six-coordinate Na atom adopts a distorted octa­hedral coordination. In the crystal structure, inter­molecular N—H⋯I and O—H⋯N hydrogen bonds link the mol­ecules into a two-dimensional network

    Role of phosphatase of regenerating liver 1 (PRL1) in spermatogenesis

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    The PRL phosphatases are oncogenic when overexpressed but their in vivo biological function is less well understood. Previous gene deletion study revealed a role for PRL2 in spermatogenesis. We report here the first knockout mice lacking PRL1, the most related homolog of PRL2. We found that loss of PRL1 does not affect spermatogenesis and reproductive ability of male mice, likely due to functional compensation by the relatively higher expression of PRL2 in the testes. However, PRL1-/-/PRL2+/- male mice show testicular atrophy phenotype similar to PRL2-/- mice. More strikingly, deletion of one PRL1 allele in PRL2-/- male mice causes complete infertility. Mechanistically, the total level of PRL1 and PRL2 is negatively correlated with the PTEN protein level in the testis and PRL1+/-/PRL2-/- mice have the highest level of PTEN, leading to attenuated Akt activation and increased germ cell apoptosis, effectively halting spermatozoa production. These results provide the first evidence that in addition to PRL2, PRL1 is also required for spermatogenesis by downregulating PTEN and promoting Akt signaling. The ability of the PRLs to suppress PTEN expression underscores the biochemical basis for their oncogenic potential

    A high-throughput FRET-based assay for determination of Atg4 activity

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    Atg4 is required for cleaving Atg8, allowing it to be conjugated to phosphatidylethanolamine on phagophore membranes, a key step in autophagosome biogenesis. Deconjugation of Atg8 from autophagosomal membranes could be also a regulatory step in controlling autophagy. Therefore, the activity of Atg4 is important for autophagy and could be a target for therapeutic intervention. In this study, a sensitive and specific method to measure the activity of two Atg4 homologs in mammalian cells, Atg4A and Atg4B, was developed using a fluorescence resonance energy transfer (FRET)-based approach. Thus LC3B and GATE-16, two substrates that could be differentially cleaved by Atg4A and Atg4B, were fused with CFP and YFP at the N- and C-terminus, respectively, allowing FRET to occur. The FRET signals decreased in proportion to the Atg4-mediated cleavage, which separated the two fluorescent proteins. This method is highly efficient for measuring the enzymatic activity and kinetics of Atg4A and Atg4B under in vitro conditions. Applications of the assay indicated that the activity of Atg4B was dependent on its catalytic cysteine and expression level, but showed little changes under several common autophagy conditions. In addition, the assays displayed excellent performance in high throughput format and are suitable for screening and analysis of potential modulators. In summary, the FRET-based assay is simple and easy to use, is sensitive and specific, and is suitable for both routine measurement of Atg4 activity and high-throughput screening

    Measurement-device-independent quantum key distribution over untrustful metropolitan network

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    Quantum cryptography holds the promise to establish an information-theoretically secure global network. All field tests of metropolitan-scale quantum networks to date are based on trusted relays. The security critically relies on the accountability of the trusted relays, which will break down if the relay is dishonest or compromised. Here, we construct a measurement-device-independent quantum key distribution (MDIQKD) network in a star topology over a 200 square kilometers metropolitan area, which is secure against untrustful relays and against all detection attacks. In the field test, our system continuously runs through one week with a secure key rate ten times larger than previous result. Our results demonstrate that the MDIQKD network, combining the best of both worlds --- security and practicality, constitutes an appealing solution to secure metropolitan communications.Comment: 17 pages, 4 figure
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