249 research outputs found
Crystalline and Electronic Structures of Molecular Solid CCl: First-Principles Calculation
A molecular solid CCl with possible crystalline structures,
including the hexagonal-close-packed (hcp) phase, the face-centered cubic (fcc)
phase, and a hexagonal monolayer, is predicted in terms of first-principles
calculation within the density functional theory. The stable structures are
determined from the total-energy calculations, where the hcp phase is uncovered
more stable than the fcc phase and the hexagonal monolayer in energy per
molecule. The energy bands and density of states for hcp and fcc
CCl are presented. The results show that CCl%
molecules can form either a hcp or fcc indirect-gap band insulator or an
insulating hexagonal monolayer.Comment: 5 pages, 6 figure
Synthese und strukturelle Charakterisierung von Bis(pentamethylcyclopentadienylmolybdän-μ-sulfido)-Komplexen mit μ,η1-SSR-Liganden(= SYNTHESIS AND STRUCTURAL CHARACTERIZATION OF BIS(PENTAMETHYLCYCLOPENTADIENYLMOLYBDENUM-MU-SULFIDO) COMPLEXES WITH MU,ETA-1-SSR LIGANDS)
The reaction of Cp2*Mo2S4I2(Cp* = eta(5)-C5Me5) with two equivalents of NaSR (R = Me, (i)Pr, (t)Bu, Ph) gives the complexes Cp2*Mo2(mu,eta(1)-SSR)2(mu-S)2 (2a-d) in nearly quantitative yields. The compounds have been investigated spectroscopically and in the case of R = Ph (2d) by means of X-ray diffraction analysis. The results show the presence of two eta(1)-PhSS- bridges (d(s-s) 2.139(2) angstrom) and that exclusively the trans-isomer is formed. All sulfur atoms lie in one plane perpendicular to the Mo-Mo axis and bisecting it
A rapid, simple, and low-blank pumped ion-exchange column chromatography technique for boron purification from carbonate and seawater matrices
Funding: This work is supported by the European Research Council under the European Union's Horizon 2020 research and innovation program (Grant 805246) to J.W.B.R., H.J., a Natural Environmental Research Council (NERC)-IAPETUS2 Doctoral Training Programme (DTP) Studentship to NE/S007431/1 C.X., a NERC-IAPETUS DTP Studentship NE/RO12253/1 to M.T., a Leverhulme Trust Early Career Fellowship ECF-2023-199 to H.J., a NERC UK IODP grant NE/P000878/1 to S.B. and S.N., and a Taiwanese MOST Grant 111-2116M-002-032-MY3 to S.N.Boron isotope ratios (δ11B) are used across the Earth Sciences and are increasing analyzed by Multi-Collector Inductively Coupled Plasma Mass Spectrometry (MC-ICPMS). Accurate δ11B MC-ICPMS analysis requires boron purification from the sample matrix using ion-exchange column chromatography. However, the traditional gravity-drip column method is time-consuming and prone to airborne contamination due to its long duration and open resin surface. To address these issues, we designed a novel, simple, and reliable column chromatography technique called “peri-columns.” This method uses a peristaltic pump to generate vacuum on a commonly used column set up. This method uses sealed collection beakers and does not require solutions to pass through pump tubing, minimizing contamination. The duration is reduced by eight-fold, processing 12 samples in just 1.5 hr. It also yields low and consistent total procedural blanks, averaging 11 pg. The efficiency and efficacy of this method were tested by repeated boron purification from calcium carbonate and high-sodium matrices with international and in-house reference materials. The results matched those obtained using the gravity column method and fell within our laboratory long-term and international certified values. The mean δ11B and 2SD (standard deviation) of repeatedly processed NIST 8301f were 14.57 ± 0.26‰ (n = 31), NIST 8301c was 24.19 ± 0.33‰ (n = 10), STAiG-F1 was 16.20 ± 0.26‰ (n = 13), and seawater was 39.52 ± 0.32‰ (n = 10). All the components of our techniques are commercially available, and it is easily adaptable to other laboratories and isotope systems.Publisher PDFPeer reviewe
A simple, low-blank batch purification method for high-precision boron isotope analysis
This work was supported by NERC IAPETUS PhD Studentships NE/RO12253/1 to M.T., J.C.B. and E.L., an IAPETUS2 PhD Studentship NE/S007431/1 to C.X.; S.N. was supported by the MOST 111-2116M-002-032-MY3 Grant; J.W.B.R acknowledges support from NERC (Grant NE/N011716/1) and from the European Research Council under the European Union's Horizon 2020 research and innovation program (Grant agreement 805246).Boron (B) isotopes are widely used in the Earth sciences to trace processes ranging from slab recycling in the mantle to changes in ocean pH and atmospheric CO2. Boron isotope analysis is increasingly achieved by multi-collector inductively coupled plasma mass spectrometry, which requires separation of B from the sample matrix. Traditional column chromatography methods for this separation have a well-established track record but are time consuming and prone to contamination from airborne blank. Here, we present an extensive array of tests that establish a novel method for B purification using a batch method. We discuss the key controls and limitations on sample loading, matrix removal and B elution including sample volume, ionic strength, buffer to acid ratio and elution volume, all of which may also help optimize column-based methods. We find consistent, low procedural blanks of 10 ± 16 pg and excellent reproducibility: 10 ng NIST RM 8301 foram [8301f] yields 14.58 ± 0.11‰ 2SD n = 15; 2.5 ng 8301f yields 14.60 ± 0.19‰ 2SD, n = 31; and overall long term 2SD on n = 218 samples pooling different sample sizes yields 14.62 ± 0.21‰ 2SD. This method also offers significant advantages in throughput, allowing the processing of 24 samples in ∼5 hr. This boron batch method thus provides a fast, reproducible, low-blank method for purification of boron for high precision isotopic analyses.Peer reviewe
Missense mutations in Desmocollin-2 N-terminus, associated with arrhythmogenic right ventricular cardiomyopathy, affect intracellular localization of desmocollin-2 in vitro
<p>Abstract</p> <p>Background</p> <p>Mutations in genes encoding desmosomal proteins have been reported to cause arrhythmogenic right ventricular cardiomyopathy (ARVC), an autosomal dominant disease characterised by progressive myocardial atrophy with fibro-fatty replacement.</p> <p>We screened 54 ARVC probands for mutations in desmocollin-2 (<it>DSC2</it>), the only desmocollin isoform expressed in cardiac tissue.</p> <p>Methods</p> <p>Mutation screening was performed by denaturing high-performance liquid chromatography and direct sequencing.</p> <p>To evaluate the pathogenic potentials of the <it>DSC2 </it>mutations detected in patients affected with ARVC, full-length wild-type and mutated cDNAs were cloned in eukaryotic expression vectors to obtain a fusion protein with green fluorescence protein (GFP); constructs were transfected in neonatal rat cardiomyocytes and in HL-1 cells.</p> <p>Results</p> <p>We identified two heterozygous mutations (c.304G>A (p.E102K) and c.1034T>C (p.I345T)) in two probands and in four family members. The two mutations p.E102K and p.I345T map to the N-terminal region, relevant to adhesive interactions.</p> <p>In vitro functional studies demonstrated that, unlike wild-type DSC2, the two N-terminal mutants are predominantly localised in the cytoplasm.</p> <p>Conclusion</p> <p>The two missense mutations in the N-terminal domain affect the normal localisation of DSC2, thus suggesting the potential pathogenic effect of the reported mutations. Identification of additional DSC2 mutations associated with ARVC may result in increased diagnostic accuracy with implications for genetic counseling.</p
The Methyl-CpG Binding Proteins Mecp2, Mbd2 and Kaiso Are Dispensable for Mouse Embryogenesis, but Play a Redundant Function in Neural Differentiation
The precise molecular changes that occur when a neural stem (NS) cell switches from a programme of self-renewal to commit towards a specific lineage are not currently well understood. However it is clear that control of gene expression plays an important role in this process. DNA methylation, a mark of transcriptionally silent chromatin, has similarly been shown to play important roles in neural cell fate commitment in vivo. While DNA methylation is known to play important roles in neural specification during embryonic development, no such role has been shown for any of the methyl-CpG binding proteins (Mecps) in mice.. No evidence for functional redundancy between these genes in embryonic development or in the derivation or maintenance of neural stem cells in culture was detectable. However evidence for a defect in neuronal commitment of triple knockout NS cells was found.Although DNA methylation is indispensable for mammalian embryonic development, we show that simultaneous deficiency of three methyl-CpG binding proteins genes is compatible with apparently normal mouse embryogenesis. Nevertheless, we provide genetic evidence for redundancy of function between methyl-CpG binding proteins in postnatal mice
Trochanteric fractures in the elderly: the influence of primary hip arthroplasty on 1-year mortality
Acromioclavicular joint reconstruction with coracoacromial ligament transfer using the docking technique
<p>Abstract</p> <p>Background</p> <p>Symptomatic Acromioclavicular (AC) dislocations have historically been surgically treated with Coracoclavicular (CC) ligament reconstruction with transfer of the Coracoacromial (CA) ligament. Tensioning the CA ligament is the key to success.</p> <p>Methods</p> <p>Seventeen patients with chronic, symptomatic Type III AC joint or acute Type IV and V injuries were treated surgically. The distal clavicle was resected and stabilized with CC ligament reconstruction using the CA ligament. The CA ligament was passed into the medullary canal and tensioned, using a modified 'docking' technique. Average follow-up was 29 months (range 12–57).</p> <p>Results</p> <p>Postoperative ASES and pain significantly improved in all patients (p = 0.001). Radiographically, 16 (94%) maintained reduction, and only 1 (6%) had a recurrent dislocation when he returned to karate 3 months postoperatively. His ultimate clinical outcome was excellent.</p> <p>Conclusion</p> <p>The docking procedure allows for tensioning of the transferred CA ligament and healing of the ligament in an intramedullary bone tunnel. Excellent clinical results were achieved, decreasing the risk of recurrent distal clavicle instability.</p
Laser excitation of the 1s-hyperfine transition in muonic hydrogen
The CREMA collaboration is pursuing a measurement of the ground-state
hyperfine splitting (HFS) in muonic hydrogen (p) with 1 ppm accuracy by
means of pulsed laser spectroscopy to determine the two-photon-exchange
contribution with relative accuracy. In the proposed
experiment, the p atom undergoes a laser excitation from the singlet
hyperfine state to the triplet hyperfine state, {then} is quenched back to the
singlet state by an inelastic collision with a H molecule. The resulting
increase of kinetic energy after the collisional deexcitation is used as a
signature of a successful laser transition between hyperfine states. In this
paper, we calculate the combined probability that a p atom initially in
the singlet hyperfine state undergoes a laser excitation to the triplet state
followed by a collisional-induced deexcitation back to the singlet state. This
combined probability has been computed using the optical Bloch equations
including the inelastic and elastic collisions. Omitting the decoherence
effects caused by {the laser bandwidth and }collisions would overestimate the
transition probability by more than a factor of two in the experimental
conditions. Moreover, we also account for Doppler effects and provide the
matrix element, the saturation fluence, the elastic and inelastic collision
rates for the singlet and triplet states, and the resonance linewidth. This
calculation thus quantifies one of the key unknowns of the HFS experiment,
leading to a precise definition of the requirements for the laser system and to
an optimization of the hydrogen gas target where p is formed and the laser
spectroscopy will occur.Comment: 21 pages, 4 figure
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