A terahertz vibrational molecular clock with systematic uncertainty at the 10−1410^{-14} level

Neutral quantum absorbers in optical lattices have emerged as a leading platform for achieving clocks with exquisite spectroscopic resolution. However, the studies of these clocks and their systematic shifts have so far been limited to atoms. Here, we extend this architecture to an ensemble of diatomic molecules and experimentally realize an accurate lattice clock based on pure molecular vibration. We evaluate the leading systematics, including the characterization of nonlinear trap-induced light shifts, achieving a total systematic uncertainty of $4.6\times10^{-14}$. The absolute frequency of the vibrational splitting is measured to be 31 825 183 207 592.8(5.1) Hz, enabling the dissociation energy of our molecule to be determined with record accuracy. Our results represent an important milestone in molecular spectroscopy and THz-frequency standards, and may be generalized to other neutral molecular species with applications for fundamental physics, including tests of molecular quantum electrodynamics and the search for new interactions.Comment: 17 pages, 8 figure

In vitro inhibition of aeromonas hydrophila growth by ethanolic extracts obtained from leaves of various ficus species (Moraceae)

рыбы, болезни рыб, инфекционные болезни рыб, аэромоноз, аэромонады, ингибирование роста, питательные среды, этанольные экстракты, фикус, листь

Changes in cognitive functions in a girl with severe acquired hypothyroidism in comparison to the healthy twin sister

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Phytosulfokine stimulates cell divisions in sugar beet (Beta vulgaris L.) mesophyll protoplast cultures

The aim of this work was to improve plating efficiency of sugar beet mesophyll protoplast cultures. Preliminary experiments showed that cultures of good quality, viable protoplasts were obtained in rich media based on the Kao and Michayluk formulation and with the calcium alginate as an embedding matrix. Nevertheless, in these cultures cell divisions were either not observed or very seldom confirming earlier reported recalcitrance of sugar beet protoplasts. The recalcitrant status of these cultures was reversed upon application of exogenous phytosulfokine (PSK)—a peptidyl plant growth factor. The highest effectiveness of PSK was observed at 100 nM concentration. Plating efficiencies obtained in the presence of PSK reached approximately 20% of the total cultured cells. The stimulatory effect of phytosulfokine was observed for all tested breeding stocks of sugar beet. Our data indicate that PSK is a powerful agent able to overcome recalcitrance of plant protoplast cultures

High Speed Two-Photon Imaging of Calcium Dynamics in Dendritic Spines: Consequences for Spine Calcium Kinetics and Buffer Capacity

Rapid calcium concentration changes in postsynaptic structures are crucial for synaptic plasticity. Thus far, the determinants of postsynaptic calcium dynamics have been studied predominantly based on the decay kinetics of calcium transients. Calcium rise times in spines in response to single action potentials (AP) are almost never measured due to technical limitations, but they could be crucial for synaptic plasticity. With high-speed, precisely-targeted, two-photon point imaging we measured both calcium rise and decay kinetics in spines and secondary dendrites in neocortical pyramidal neurons. We found that both rise and decay kinetics of changes in calcium-indicator fluorescence are about twice as fast in spines. During AP trains, spine calcium changes follow each AP, but not in dendrites. Apart from the higher surface-to-volume ratio (SVR), we observed that neocortical dendritic spines have a markedly smaller endogenous buffer capacity with respect to their parental dendrites. Calcium influx time course and calcium extrusion rate were both in the same range for spines and dendrites when fitted with a dynamic multi-compartment model that included calcium binding kinetics and diffusion. In a subsequent analysis we used this model to investigate which parameters are critical determinants in spine calcium dynamics. The model confirmed the experimental findings: a higher SVR is not sufficient by itself to explain the faster rise time kinetics in spines, but only when paired with a lower buffer capacity in spines. Simulations at zero calcium-dye conditions show that calmodulin is more efficiently activated in spines, which indicates that spine morphology and buffering conditions in neocortical spines favor synaptic plasticity