Ionic liquids form ideal solutions

An understanding of the activity of a solute in solution is vital for utilising the full potential of a reactive species. In this work we determine the activity of metal salts in a variety of ionic liquids. Some solutions behave like classical non-polar solvents whereas other are practically ideal solutions up to 1 mol kg(-1) which allows standard redox potentials to be determined.     

High-throughput tools for the study of protein-nanostructured surface interaction

The aim of this review is to describe and to analyze the ingredients that are necessary in order to develop a robust and effective experimental approach for the high-throughput characterization of protein-nanostructured surface interaction. In the first part of this paper we review the nanostructured surface synthesis methods that are potentially able to create nanostructured inorganic surface libraries. In the second part, we address another fundamental aspect consisting in the availability of high-throughput proteins detection methods. We describe in details new emerging analytical tools compatible with nanostructured surfaces, analyzing different possible strategies, depending on the objective of the experiment and on the library format.     

Warped electroweak breaking without custodial symmetry

We propose an alternative to the introduction of an extra gauge (custodial) symmetry to suppress the contribution of KK modes to the T   parameter in warped theories of electroweak breaking. The mechanism is based on a general class of warped 5D metrics and a Higgs propagating in the bulk. The metrics are nearly AdS in the UV region but depart from AdS in the IR region, towards where KK fluctuations are mainly localized, and have a singularity outside the slice between the UV and IR branes. This gravitational background is generated by a bulk stabilizing scalar field which triggers a natural solution to the hierarchy problem. Depending on the model parameters, gauge-boson KK modes can be consistent with present bounds on EWPT for mKK?1 TeV$m_{\mathit{KK}}?1\text{TeV}$ at 95% CL. The model contains a light Higgs mode which unitarizes the four-dimensional theory. The reduction in the precision observables can be traced back to a large wave function renormalization for this mode.     

Electrically detected electron-spin-echo envelope modulation: a highly sensitive technique for resolving complex interface structures

We show that the electrical detection of electron-spin-echo envelope modulation (ESEEM) is a highly sensitive tool to study interfaces. Taking the Si/SiO2 interface defects in phosphorus-doped crystalline silicon as an example, we find that the main features of the observed echo modulation pattern allow us to develop a microscopic model for the dangling-bond-like P(b0) center by comparison with the results of ab initio calculations. The ESEEM spectrum is found to be far more sensitive to the defect characteristics than the spectrally resolved hyperfine splitting itself.     

Isoprenoid quantitation in human brain tissue: a validated HPLC–fluorescence detection method for endogenous farnesyl- (FPP) and geranylgeranylpyrophosphate (GGPP)

Farnesyl- and geranylgeranylpyrophosphate (FPP and GGPP) are isoprenoid intermediates in the mevalonate pathway. They play a crucial role in cell survival, growth and differentiation due to their attachment (isoprenylation) to small GTPases (Ras, Rho, etc.). Isoprenoid formation seems to be tightly regulated within the mevalonate pathway and its perturbation has been linked to certain diseases (e.g., cancer, Alzheimer's disease), but tissue levels are unknown. It is therefore of the utmost importance to quantify these isoprenoids in diseased tissue or in tissue after drug administration. The current work describes an isolation procedure utilizing a combination of Extrelut(R) liquid/liquid and reversed-phase solid-phase extraction (SPE) for homogenized human frontal cortex tissue. In addition, after a careful validation of an HPLC-fluorescence method, this assay allowed the determination of nanomolar concentrations of endogenous FPP and GGPP levels (4.5 and 10.6 ng/mg protein, respectively) in human brain tissue. The method is selective, precise (<15% RSD), accurate (<15% relative error) and sensitive over a linear range of 10-400 ng/mL for FPP and 50-1000 ng/mL for GGPP according to the current FDA criteria for bioanalytical method validation. Overall, this new method introduces the ability to simultaneously quantify FPP and GGPP in human brain tissue, and is potentially applicable to several other tissues and species.     

Slow complexation dynamics between linear short polyphosphates and polyallylamines: analogies with "layer-by-layer" deposits

Polyelectrolyte "complexes" have been studied for almost a century and find more and more applications in cosmetics and DNA transfection. Most of the available studies focused on the thermodynamic aspects of the "complex" formation, mainly to determine phase diagrams and the influence of diverse physicochemical aspects on the formation of "complexes", but conversely less effort has been given to the kinetics of such processes. We describe herein the "complexation" kinetics of a short linear sodium polyphosphate (PSP) with poly(allylamine hydrochloride) (PAH) in the presence of 10 mM, 0.15 M and 1 M NaCl. We find, by using a combination of physicochemical techniques, that mixtures containing a 1 to 1 molar ratio of phosphate and amino groups allow the formation of "complexes" having a few 100 nm in diameter which progressively grow to particles up to 1.5 microns in hydrodynamic diameter, the growth process being accompanied by some progressive sedimentation. During this slow aggregation kinetics, the polyelectrolytes undergo a release of counterions and the zeta potential changes from a positive value to a negative one of -20 mV which is close to the zeta potential of (PSP-PAH)(n) films deposited under identical physicochemical conditions. Even though the complexes have a negative electrophoretic mobility, they contain an equimolar amount of amino and phosphate groups. This allows us to make some assumption about the structure of such "complexes" and to compare them with other published structures. We will also compare them with the aggregates found during the "layer-by-layer" deposition of the same species under the same conditions.     

Self-compression of millijoule pulses to 7.8 fs duration in a white-light filament

We demonstrate a novel technique for pulse compression of few-millijoule pulses with shorter than 10 fs duration. Our technique relies on spectral broadening in a white-light filament generated in a noble gas. In this filament we observe self-compression of 45 fs pulses down to below 8 fs duration without the need for any additional dispersion compensation. Using input pulses of 5 mJ, we generate compressed pulses with up to 3.8 mJ pulse energy. Therefore this method is much more efficient than previously demonstrated compression schemes. The generated peak powers of more than 100 GW at a kilohertz repetition rate open up a perspective for compression of few-cycle pulses with energies well beyond the capacity of hollow-fiber compressors.     

Evaluation of whole-genome amplification of low-copy-number DNA in chimerism analysis after allogeneic stem cell transplantation using STR marker typing

Whole-genome DNA amplification (WGA) is a promising method that generates large amounts of DNA from samples of limited quantity. We investigated the accuracy of a multiplex PCR approach to WGA over STR loci. The amplification bias within a locus and over all analyzed loci was investigated in relation to the amount of template in the WGA reaction, the specific STR locus, and allele length. We observed reproducible error-free STR profiles with 10 ng down to 1 ng of DNA template. The amplification deviation at a locus and between loci was within the intra-method reproducibility. WGA is the method of choice for amplifying nanogram amounts of genomic DNA for different applications. We detected unbalanced STR amplifications at one locus and between loci, allelic drop-outs, and additional alleles after WGA of low-copy-number DNA. We found that the high number of drop-outs and drop-ins could be eradicated using pooled DNA from separate WGA reactions even with as little as 100 pg of starting template. Nevertheless, the quality of the results was still not sufficient for use in routine chimerism analysis of limited specific cell populations after allogeneic stem cell transplantation.