The study of the changes in the thermal properties of <Emphasis Type="Italic">Labeo rohita</Emphasis> bones due to arsenic exposure

The paper presents the changes in the thermal properties of control, arsenic exposed and DMSA treated Labeo rohita bones by using thermo analytical techniques. The result shows that the mass loss due to the thermal decomposition occurs in three distinct steps due to loss of water, organic and inorganic materials. The arsenic exposed bones present a different thermal behaviour compared to the control bones. The residue masses are increased due to arsenic exposure, while the DMSA treatment reduces the residue mass level. These thermal characteristics can be used as a qualitative method to check the metal accumulation in samples.     

pH-triggered assembly of gold nanorods

The self-assembly of surfactant-protected gold nanorods (aspect ratio 3.3 +/- 0.3, 20.6 +/- 5.5 nm width, and 67.5 +/- 9.0 nm length) into ordered structures using adipic acid is presented. As made, the gold nanorods are coated with cationic surfactant, which gives them a net positive charge in aqueous solution. The pH-dependent assembly is directed by electrostatic interactions between the positively charged nanorods and negatively charged, deprotonated adipic acid. Absorption spectra and light scattering measurements of these nanorods suggest that aggregation is initiated in solution in the presence of adipic acid at pH 7-8, but not at pH 3, to form small assemblies of nanorods. Zeta potential measurements show that the assembly is significantly less positively charged in the presence of deprotonated adipic acid than when adipic acid is fully protonated.     

Micro-interferometric backscatter detection using a diode laser

Micro-interferometric backscatter detection (MIBD) is performed with a simple, folded optical train based on the interaction of a diode laser beam and a fused silica capillary tube allowing for refractive index (RI) determinations and detection of optically active molecules in small volumes. Side illumination of the capillary by a laser produces a 360° fan of scattered light that contains two sets of high contrast interference fringes. These light and dark spots are viewed on a flat plane in the direct backscatter configuration. Signal interrogation for polarimetry is based on quantifying the relative intensities (depth of modulation (DOM)) of adjacent high frequency (HF) interference fringes for polarimetry and relative fringe position for RI detection. Positional changes of the interference pattern extrema (fringes) allow for the determination of Δn at the 10⁻⁷ level or 5.3 pmol or 0.48 ng of solute. The MIBD-RI detection volume is just 5.0 nl. DOM changes allow for optical activity detection limits of 5.7 × 10⁻⁵° (mandelic acid, []²³ = −153°, and D-glucose, []²⁵ = +52.5°), and a 2σ detection limit of 7.5 × 10⁻⁴ M (D-glucose) and 1.14 × 10⁻³ M (R-mandelic acid). The probe volume of MIBD-polarimetry was 38 nl, and within the probed volume at the limit of detection, about 28.7 pmol of mandelic acid or about 43.7 pmol of D-glucose is present. Furthermore, DOM (polarimetry signal) is unchanged when a non-optically active solute is interrogated by the MIBD-polarimeter. Finally, an optical model was derived and used to evaluate the advantages and pitfalls of using diode laser for MIBD.     

Dual Electrode Ensembles with Core and Shell Nanoelectrodes for Dopamine Sensing Applications

This paper presents the fabrication of dual electrode ensembles for electrochemical sensing of dopamine. A new dual electrode ensemble consists of vertically aligned core nanowire electrodes and a shell electrode with a hemi‐cylindrical nanocavity structure and submicron inter‐electrode spacing between the two working electrodes. By using a 3‐dimensional cavity structure of two working electrodes, collection efficiency in redox cycling of dopamine is enhanced. Initial measurement results show the ability to detect 200 μM concentration of dopamine with 69% collection efficiency on a dual electrode ensemble.     

Quantitative determination of pravastatin and its metabolite 3α‐hydroxy pravastatin in plasma and urine of pregnant patients by LC‐MS/MS

This report describes the development and validation of a chromatography/tandem mass spectrometry method for the quantitative determination of pravastatin and its metabolite (3α‐hydroxy pravastatin) in plasma and urine of pregnant patients under treatment with pravastatin, as part of a clinical trial. The method includes a one‐step sample preparation by liquid–liquid extraction. The extraction recovery of the analytes ranged between 93.8 and 99.5% in plasma. The lower limits of quantitation of the analytes in plasma samples were 0.106 ng/mL for pravastatin and 0.105 ng/mL for 3α‐hydroxy pravastatin, while in urine samples they were 19.7 ng/mL for pravastatin and 2.00 ng/mL for 3α‐hydroxy pravastatin. The relative deviation of this method was <10% for intra‐ and interday assays in plasma and urine samples, and the accuracy ranged between 97.2 and 106% in plasma, and between 98.2 and 105% in urine. The method described in this report was successfully utilized for determining the pharmacokinetics of pravastatin in pregnant patients enrolled in a pilot clinical trial for prevention of preeclampsia. Copyright © 2015 John Wiley & Sons, Ltd.     

Quantitative determination of famotidine in human maternal plasma,umbilical cord plasma and urine using high‐performance liquid chromatography–mass spectrometry

Liquid chromatography with electrospray ionization mass spectrometry for the quantitative determination of famotidine in human urine, maternal and umbilical cord plasma was developed and validated. The plasma samples were alkalized with ammonium hydroxide and extracted twice with ethyl acetate. The extraction recovery of famotidine in maternal and umbilical cord plasma ranged from 53 to 64% and 72 to 79%, respectively. Urine samples were directly diluted with the initial mobile phase then injected into the HPLC system. Chromatographic separation of famotidine was achieved by using a Phenomenex Synergi? Hydro‐RP? column with a gradient elution of acetonitrile and 10 mm ammonium acetate aqueous solution (pH 8.3, adjusted with ammonium hydroxide). Mass spectrometric detection of famotidine was set in the positive mode and used a selected ion monitoring method. Carbon‐13‐labeled famotidine was used as internal standard. The calibration curves were linear (r² > 0.99) in the concentration ranges of 0.631–252 ng/mL for umbilical and maternal plasma samples and 0.075–30.0 µg/mL for urine samples. The relative deviation of method was <14% for intra‐ and inter‐day assays, and the accuracy ranged between 93 and 110%. The matrix effect of famotidine in human urine, maternal and umbilical cord plasma was less than 17%. Copyright © 2013 John Wiley & Sons, Ltd.     

On distribution by rank of bases for vector spaces of matrices over a finite field

Let F^m×n_q denote the vector space of all m×n matrices over the finite field F_q of order q, and let $\text{B}\text{=(A}{}_1\text{,A}{}_2\text{,…,A}{}_{\mathrm{mn}}\text{)}$ denote an ordered basis for F^m×n_q. If the rank of A_i is r_i,i=1,2,…,mn, then $\text{B}$ is said to have rank (r₁,r₂,…,r_mn), and the number of ordered bases of F^mxn_q with rank (r₁,r₂,…,r_mn is denoted by N_q(r₁, r₂,…,r_mn). This paper determines formulas for the numbers N_q(r₁,r₂,…,r_mn) for the case m=n=2, q arbitrary, and while some of the techniques of the paper extend to arbitrary m and n, the general formulas for the numbers N_q(r₁,r₂,…,r_mn) seem quite complicated and remain unknown. An idea on a possible computer attack which may be feasible for low values of m and n is also discussed.