Utilization of low-cost sorbent for removal and separation of 134Cs, 60Co and 152+154Eu radionuclides from aqueous solution

Eggshell material was used as low-cost and eco-friendly biosorbent for removal of ¹³⁴Cs, ⁶⁰Co and ^152+154Eu radionuclides from aqueous solution. The eggshell material was calcined at 500 and 800 °C, and then characterized. Comparative studies on the natural and calcined eggshell for sorption of the three radionuclides were carried out. It was found that, the uptake is in the order: Eu(III) > Co(II) > Cs(I). Further, column chromatography was used in separation of ¹³⁴Cs, ⁶⁰Co and ^152+154Eu using 0.15, 0.2 and 0.5 mol/l nitric acid, respectively. Eggshell material can be considered as a promising material for separation of radionuclides from radioactive waste solution.     

Determination of neurotransmitters and their metabolites using one- and two-dimensional liquid chromatography with acidic potassium permanganate chemiluminescence detection

High-performance liquid chromatography with chemiluminescence detection based on the reaction with acidic potassium permanganate and formaldehyde was explored for the determination of neurotransmitters and their metabolites. The neurotransmitters norepinephrine and dopamine were quantified in the left and right hemispheres of rat hippocampus, nucleus accumbens and prefrontal cortex, and the metabolites vanillylmandelic acid, 3,4-dihydrophenylacetic acid, 5-hydroxyindole-3-acetic acid and homovanillic acid were identified in human urine. Under optimised chemiluminescence reagent conditions, the limits of detection for these analytes ranged from 2.5?×?10^?8 to 2.5?×?10^?7 M. For the determination of neurotransmitter metabolites in urine, a two-dimensional high-performance liquid chromatography (2D-HPLC) separation operated in heart-cutting mode was developed to overcome the peak capacity limitations of the one-dimensional separation. This approach provided the greater separation power of 2D-HPLC with analysis times comparable to conventional one-dimensional separations. Figure

2D-HPLC separation and permanganate chemiluminescence detection of neurotransmitter metabolites     

Stereoselective separation and pharmacokinetic dissipation of the chiral neonicotinoid sulfoxaflor in soil by ultraperformance convergence chromatography/tandem mass spectrometry

Ultraperformance convergence chromatography/tandem triple quadrupole mass spectrometry (UPC²-MS/MS) is a novel tool in separation science that combines the advantages of supercritical fluid chromatography with ultraperformance liquid chromatography/MS/MS technology. The use of nontoxic CO₂ fluid and a postcolumn additive to complement MS/MS allows better control of analyte retention for chiral separation and high-sensitivity determination with different chiral stationary phases. This paper reports the stereoselective separation and determination of the chiral neonicotinoid sulfoxaflor in vegetables and soil by UPC²-MS/MS. Baseline resolution (Rs?≥?1.56) of and high selectivity (LOQ?≤?1.83 μg/kg) for the four stereoisomers were achieved by postcolumn addition of 1 % formic acid–methanol to a Chiralpak IA-3 using CO₂/isopropanol/acetonitrile as the mobile phase at 40 °C, 2,500 psi, and for 6.5 min in electrospray ionization positive mode. Rearranged Van’t Hoff equations afforded the thermodynamic parameters ΔH ^ο and ΔS ^ο, which were analyzed to promote understanding of the enthalpy-driven separation of sulfoxaflor stereoisomers. The interday mean recovery, intraday repeatability, and interday reproducibility varied from 72.9 to 103.7 %, from 1.8 to 9.2 %, and from 3.1 to 9.4 %, respectively. The proposed method was used to study the pharmacokinetic dissipation of sulfoxaflor stereoisomers in soil under greenhouse conditions. The estimated half-life ranged from 5.59 to 6.03 d, and statistically nonsignificant enantioselective degradation was observed. This study not only demonstrates that the UPC²-MS/MS system is an efficient and sensitive method for sulfoxaflor stereoseparation, but also provides the first experimental evidence of the pharmacokinetic dissipation of sulfoxaflor stereoisomers in the environment. Graphical Abstract

Chemical structure and UPC²-MS/MS separation chromatogram of sulfoxaflor. (* stereogenic center)     

Studies on the selectivity of Na+ separation on specially prepared hydrated antimony pentoxide

The selectivity of Na⁺ separation on especially prepared hydrated antimony pentoxide (HAP) was studied with respect to trace elements. For this purpose NaCl samples, doped with 0.5 μg each of altogether 21 selected elements in form of suitable neutron activated compounds, were in relation to practice subjected to column experiments. In some cases trace elements were used in different oxidation states. Considered were elements which are of particular interest for neutron activation analysis. With simultaneous retention of Na⁺ (DK≥10⁸) Cs, Ba, Sc, La, Ce, Eu, Cr, Mo, Mn, Co, Cu, Ag, Au, Zn, Cd, Hg, and Sb are completely eluted from the HAP column, using 7.5N HCl, whereby Cs and to some extent Ba and Sc in comparison to the elements mentioned above required a higher elution volume. Rb, Se and As on the contrary were almost quantitatively retained on HAP column, W partly as WO ₄ ^2? . The scope of validity of the results will be discussed.     

Routine quality control of11C-labelled radiopharmaceuticals by high pressure liquid chromatography

Radio high pressure liquid chromatography (radio-HPLC) is the method of choice for quality control of radiopharmaceuticals labelled with short lived isotopes. Our preparations of “no carrier added”¹¹C-labelled palmitic acid and L-methionine are both designed to end with a HPLC separation on either silica gel or C-18 reversed phase material. Since the crude reaction mixtures contain milligram amounts of inactive substrate materials, both separations must be carried out at preparative scale. Nevertheless they are performed in less than 10 min. The most critical factor for the separation of¹¹C-palmitic acid from the main by-product pentadecane is the solvent composition: while the¹¹C-L-methionine separation is especially sensitive to pH variations.     

Tracer scale solvent extraction separation of tantalum from niobium using di-(2-ethylhexyl)-phosphoric acid as extractant

A simple solvent extraction procedure for the efficient separation of the radioactive tracers⁹⁵Nb and¹⁸²Ta from each other in a mixture using di-(2-ethylhexyl)phosphoric acid (HDEHP) as extractant is described. Tantalum was found to be quantitatively extracted from an aqueous madium, which is 1.6N in HCl and 10^?2 M in oxalic acid, with a HDEHP solution of 0.1 M concentration. Extractabilities of both niobium and tantalum in mineral acids like HCl, H₂SO₄ and HNO₃ and in some organic acids like oxalic, citric, etc., in HDEHP under the experimental conditions were also studied. The reliability of the separation procedure was verified further by γ-ray spectrometry.     

Separation of tin from some metals by extraction chromatography

Much attention has been devoted to Sn (IV) strongly retained on the TBP-Daiflon column from 2M HCl in extraction chromatography. The separations of Sn?Cu, Zn, As, Cd, Sb, Pb,¹¹³Sn-¹²⁵Sb,¹¹³Sn-^113mIn (^113mIn milking) and Sn?Hg?Fe were successfully achieved without any contamination. In the separations, except for the last, only tin was retained separately on the column upon passing the mixed solution. The daughter indium was eluted with 0.5M HCl. In the last separation, iron was eluted with 0.5 M HCl, tin with 0.1M HCl and mercury with 2M HNO₃, for these metals retained on the column. Radioactive tracers for tin, iron, mercury and antimony were used.     

The Development and Validation of a Stability-Indicating UHPLC-DAD Method for Determination of Perindopril l-Arginine in Bulk Substance and Pharmaceutical Dosage Form

A stability-indicating ultra-high-performance liquid chromatography (UHPLC) method with a diode array detector was developed and validated for the determination of cis/trans isomers of perindopril l-arginine in bulk substance and pharmaceutical dosage form. The separation was achieved on a Poroshell 120 Hilic (4.6 × 150 mm, 2.7 µm) column using a mobile phase composed of acetonitrile–0.1 % formic acid (20:80 v/v) at a flow rate of 1 mL min^?1. The injection volume was 5.0 µL and the wavelength of detection was controlled at 230 nm. The selectivity of the UHPLC-DAD method was confirmed by determining perindopril l-arginine in the presence of degradation products formed during acid–base hydrolysis and oxidation as well as degradation in the solid state, at an increased relative air humidity and in dry air. The method’s linearity was investigated in the ranges 0.40–1.40 µg mL^?1 for isomer I and 0.40–2.40 µg mL^?1 for isomer II of perindopril l-arginine. The UHPLC-DAD method met the precision and accuracy criteria for the determination of the isomers of perindopril l-arginine. The limits of detection and quantitation were 0.1503 and 0.4555 µg mL^?1 for isomer I and 0.0356 and 0.1078 µg mL^?1 for isomer II, respectively.     

Isolation and alpha-particle spectrometric determination of238Pu and239,240Pu in sediments

A simple method is described for the isolation and determination of plutonium isotopes in sediments. The method involves leaching of sample with nitric acid and subsequent separation of plutonium on an anion-exchange column. Major matrix elements and several potential radiochemical interferences are removed during 8M HNO₃ sample loading on the column. Thorium is removed by thorough washing with 10M HCl. Plutonium (IV) is eluted with 4M HCl. Source for alpha-particle spectrometry is prepared by LaF₃ coprecipitation technique at which stage a complete separation from uranium(VI) is also achieved. The entire analytical procedure is completed in about two days.     

Chiral Separation of 4-Iminoflavan Derivatives on Several Polysaccharide-Based Chiral Stationary Phases by HPLC

The HPLC enantiomeric separation of seven 4-iminoflavans was successfully accomplished in the normal phase mode using six polysaccharide-based chiral stationary phases namely, Chiralcel^®OD-H, Chiralcel^®OD, Chiralcel^®OJ, Chiralpak^®AD, Chiralpak^®IA and Chiralpak^®IB under normal and polar organic phase modes. The resolution depended on nature and concentration of alcoholic modifier. The results demonstrate clearly that the chromatographic system based on the coated and immobilized type Chiralpak^®IB and Chiralcel^®OD-H CSPs provide a powerful analytical tool for enantiomeric separation of all the 4-iminoflavans used in this study.     

A generator for preparation of carrier-free224Ra

The construction of a dynamic generator for the separation of carrier-free²²⁴Ra is described. The mother²²⁸Th was extracted on the top of the column with di-(2-ethylhexyl)phosphoric acid on hydrophobized Chromosorb W DMCS. The function of the generator was checked during 6 months by measuring the decontamination of²²⁴Ra from²²⁸Th. Simultaneously the yield of²²⁴Ra was determined as a function of the HCl concentration and of the means of milking. The best results were obtained with 0.01–0.1M HCl; the yield was about 75% of the theoretical value, and the²²⁴Ra contained less than 0.01% of²²⁸Th.     

The generator production of172Lu from172Hf for limited nuclear medicine research

A solvent extraction system has been developed for the separation of¹⁷²Lu from its long-lived¹⁷²Hf parent. The parent-daughter pair in equilibrium is maintained in a solution of HDEHP, and the heavy lanthanide daughter is extracted into 9M HCl. The separation factor for this generator is approximately 10⁴. The rare-earth activity so obtained is proposed for compound labelling research and animal biodistribution studies in nuclear medicine.     

Synthesis of the bifuncttonal dinucleotide AMP-ATP and its application in general ligand affinity chromatography

A new AMP derivative substituted with spacer arms both at position N⁶ and C8 of the adenine moiety was synthesized and immobilized to Sepharose. To the immobilized ligand was subsequently coupled C8-substituted ATP in a solid-phase synthesis fashion yielding the bifunctional general ligand AMP-ATP. This affinity material was used in the separation of two major groups of enzymes, dehydrogenases and kinases. It was found that on passage of crude homogenates obtained from mouse kidney through the affinity column, several dehydrogenases and kinases were bound, which could be eluted separately using pulses of NADH and ATP, respectively. In the fractions obtained on NADH elution, lactate dehydrogenase, malate dehydrogenase, and α-glycerol phosphate dehydrogenase were found, whereas ATP eluted 3-phosphoglyceric acid kinase, pyruvate kinase, and aldolase.     

Chemical separation of molybdenum from uranium and fission product nuclides

A very rapid method for the separation of molybdenum(VI) from neutron irradiated uranium and its fission products is described. The procedure is based on the selective extraction of molybdenum(VI) by a 0.1M solution of 2-hexylpyridine in benzene from 4M HCl+0.04M KSCN. Decontamination factors were estimated to be >10⁴ for the radionuclides of niobium, zirconium, ruthenium, lanthanum, cerium, promethium, yttrium, strontium and barium.     

Using amino acids for the chromatofocusing of metal ions on silica with bonded tetraethylenepentamine groups

Amino acid-based eluents are used for the chromatofocusing of metal ions on Tetren-SiO₂ chelating sorbent (silica with bonded tetraethylenepentamine groups) for the first time. The smoothest quasilinear pH gradients form for eluents based on glutamic and aspartic acids. The separation of Mn²⁺, Cr³⁺, Co²⁺, Ni²⁺, and Cu²⁺ is achieved.     

Simultaneous sensing of L-tyrosine and epinephrine using a glassy carbon electrode modified with nafion and CeO2 nanoparticles

An electrochemical sensor was developed and tested for detection of L-tyrosine in the presence of epinephrine by surface modification of a glassy carbon electrode (GCE) with Nafion and cerium dioxide nanoparticles. Fabrication parameters of a surfactant-assisted precipitation method were optimized to produce 2–3 nm CeO₂ nanoparticles with very high surface-to-volume ratio. The resulting nanocrystals were characterized structurally and morphologically by X-ray diffractometery (XRD), scanning and high resolution transmission electron microscopy (SEM and HR-TEM). The nanopowder is sonochemically dispersed in a Nafion solution which is then used to modify the surface of a GCE electrode. The electrochemical activity of L-tyrosine and epinephrine was investigated using both a Nafion-CeO₂ coated and a bare GCE. The modified electrode exhibits a significant electrochemical oxidation effect of L-tyrosine in a 0.2 M Britton-Robinson (B-R) buffer solution of pH 2. The electro-oxidation peak current increases linearly with the L-tyrosine concentration in the molar concentration range of 2 to 160 μM. By employing differential pulse voltammetry (DPV) for simultaneous measurements, we detected two reproducible peaks for L-tyrosine and epinephrine in the same solution with a peak separation of about 443 mV. The detection limit of the sensor (signal to noise ratio of 3) for L-tyrosine is ~90 nM and the sensitivity is 0.20 μA μM^?1, while for epinephrine these values are ~60 nM and 0.19 μA μM^?1. The sensor exhibited excellent selectivity, sensitivity, reproducibility and stability as well as a very good recovery time in real human blood serum samples.

Simultaneous electrochemical determination of L-tyrosine and epinephrine in blood plasma with Nafion-CeO₂/GCE modified electrode showing a 443 mV peak-to-peak potential difference between species oxidation peak currents.     

Purification and Characterization of Calreticulin: a Ca2+-Binding Chaperone from Sheep Kidney

Calreticulin (CRT) is a molecular chaperone with a molecular mass of 46 kDa present in the endoplasmic reticulum (ER). This protein is primarily involved in the regulation of intracellular Ca²⁺ homeostasis and Ca²⁺ storage in the ER. CRT also plays a significant role in autoimmunity and cancer. This protein contains three distinct structural domains with specialized functions. Here, we are reporting a simple procedure for the purification of CRT from mammalian kidney. To isolate CRT,  sheep kidney was crushed and kept for 12 h in the extraction buffer. The lysate was centrifuged, and supernatant was precipitated by ammonium sulphate. The precipitate of 90 % ammonium sulphate was extensively dialyzed and loaded on DEAE-Hi-Trap FF and Mono Q chromatography columns. The purity of CRT was confirmed by SDS-PAGE. Finally, the protein was identified by matrix-assisted laser desorption/ionization time of flight. The purified protein was further characterized for secondary structural elements using the far-UV circular dichroism measurements. Our purification procedure is fast and simple with high yield.     

Separation of metallic impurities from uranium by anion exchange on Dowex 1×8 resin

The separation of metallic impurities from uranium by anion exchange with a Dowex 1×8 resin has been investigated. The following elements can be quantitatively separated from 400 mg uranium using a 1 cm diameter 15 or 30 cm long column. The elements Ag, Al, Ba, Ca, Cr, Cs, K, Mg, Mn, Na, Ni, Rb, REE, Sc, Th, Ti and Y can be separated by eluting the elements with conc. HCl. Uranium is retained by the resin. Al, Ca, Cd, Co, Cr, Cu, Fe, Mg, Mn, Na, REE and V can be separated by eluting with 0.01 N H₂SO₄. Uranium is retained by the resin. Cd and Zn can be separated by first eluting uranium with 0.5 N HCl and then eluting Cd and Zn with 1 N NH₃. Hf, Zr and V can be separated by eluting with 5 N HCl but some uranium contamination is unavoidable.     

Calorimetry and thermal analysis studies on the binding of 13-phenylalkyl and 13-diphenylalkyl berberine analogs to tRNAphe

The interaction of 13- monophenylalkyl and diphenylalkyl berberine analogs with tRNA^phe has been investigated using various thermochemical techniques like thermal melting, isothermal titration calorimetry, and differential scanning calorimetry experiments. Thermal melting studies revealed that all the analogs stabilized the tRNA^phe better than berberine. The binding affinity for the analogs was of the order of 10⁵ M^?1. Calorimetry results suggested that the binding of these analogs was predominantly entropy driven with small negative enthalpy contribution to the standard molar Gibbs energy. The temperature dependence of the standard molar enthalpy changes yielded negative values of standard molar heat capacity changes for the complexation revealing substantial hydrophobic contribution in the RNA binding of these analogs. An enthalpy–entropy compensation behavior was also seen in all the systems. The diphenylalkyl analogs were found to be more effective tRNA^phe binders compared to the monophenylalkyl analogs. The utility of the present work lies in understanding the structural and energetic aspects of the interaction of these berberine analogs with tRNA, which may be useful in the development of RNA-targeted drugs.