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.     

Purification and some properties of tryptophan-5-monooxygenase from rabbit hindbrain

An affinity chromatography procedure for the rapid purification of tryptophan-5-monooxygenase from rabbit hindbrains was developed using e-aminocaproyl-D-tryptophan methyl ester-Sepharose-4B gels. The precise requirements for the optimal biospecific interaction between the affinity ligand and the ligate (enzyme) was established from a study of the effects of the variation in the length of the "spacer’’ on the affinity properties of the gel. The enzyme preparation isolated by this procedure was found to be essentially homogeneous and was characterized by a molecular weight of 200,000 ±20,000. SDS-polyacrylamide gel electrophoresis of the enzyme revealed it to be a dimer, the molecular weight of each subunit being approximately 90,000. The specific activity of the enzyme preparation is approxi-mately 7-10 times that of the crude homogenate, but a further fivefold enhancement in the specific activity could be obtained by limited proteolysis with trypsin. The extreme lability of the enzyme could be circumvented by its immobilization on activated Sepharose or by cross-linking with dimethyl suberimidate. The kinetic properties as well as the advantages of such stabilized enzyme preparations are presented.     

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.     

The Effect of O6+ and Si7+ ion beam irradiations on poly(lactide-co-glycolide) (50: 50) copolymer

Sterilization by ion beam radiations unfortunately also has a significant effect on the degradation of many polymers. The aim of present study is to examine the effect of heavy ion beam irradiation on poly(lactide-co-glycolide) (PLGA) (50: 50). The radiation effect is manifested through its degradation behavior and changes in the morphological, optical and structural properties. PLGA films are prepared by solvent casting method and subsequently irradiated with swift heavy ions O⁶⁺ and Si⁷⁺ ion with fluence in the range of 5 × 10¹⁰?1 × 10¹² ions/cm². The dominant effect on PLGA films is chain scission as evidenced by change in surface modification. Changes in optical and structural properties were analyzed by UV-Vis, XRD and FTIR spectrometric techniques. XRD technique is not responsive to degradation occurring in samples. Surface modifications caused by ion irradiations have been observed with SEM.     

Separation of methyltin species from inorganic tin,and their interactions with humates in natural waters

Tin(II) and tin(IV) are absorbed from aqueous solutions by Sephadex G-25 gel, from which they can be eluted by humates or fulvates, with which they interact more strongly. Methyltin species are not absorbed by Sephadex G-25, and so can be separated from inorganic tin. Both inorganic tin and methyltin species in natural waters at pH 7.4 can be quantitatively retained by passing through small columns of Chelex-100 resin: the methyltin species can then be washed off the resin with 4M nitric acid. Trimethyltin chloride¹¹³Sn in water scarcely interacts with fulvates, humates, kaolinite or montmorillonite but is absorbed bySphagnum peat. Dimethyltin dichloride-¹¹³Sn reacts significantly with all the above materials after 2 hours equilibration. Methyltin trichloride-¹¹³Sn interacts weakly in alkaline solutions.     

Isolation of protease B from cotton seeds

Protease B has been isolated from dormant cotton seeds by fractionation with ammonium sulfate, ion-exchange chromatography on CM-cellulose, and gel filtration through Acrilex P-10 and Sephadex G-75, with 128-fold purification. The enzyme exists in dimeric and monomeric forms. According to the results of gel filtration, their molecular weights are 72,000 and 36,000, respectively. The enzyme consists of a single polypeptide chain including sugars. The N-terminal amino acid of protease B is alanine. The enzyme possesses proteolytic activity in the pH range from 4 to 6.     

Effect of Cl substituent in the aromatic tetracycline ring on its reactivity with solvated electrons

Decomposition yields of tetracycline hydrochloride /TC.HCl/ and chlorotetracycline hydrochloride /ClTC?HCl/ in methanol solution saturated with Ar or N₂O were determined. Rate constants of the reaction e_s with some antibiotics were obtained: $$\begin{gathered} k/e_s^ - + ClTC \cdot HCl/ = 2 \cdot 49 \times 10^8 dm^3 \cdot mole^{ - 1} \cdot s^{ - 1} ; \hfill \\ k/e_s^ - + TC \cdot HCl/ = 2 \cdot 86 \times 10^8 dm^3 \cdot mole^{ - 1} \cdot s^{ - 1} \cdot \hfill \\ \end{gathered} $$ On the basis of the diffence between decomposition yields: ΔG=G_?TC.HCl^?G?ClTC.HCl′ 7-C?Cl group decomposition yield and the rate constant $$k/e_s^ - + Cl - C - 7/ = 7 \cdot 94 \times 10^8 dm^3 \cdot mole^{ - 1} \cdot s^{ - 1} $$ were determined. It was demonstrated by¹H NMR that the radical formed by degradation of 7-C?Cl group is recombined with the H atoms leading to ClTC.HCl being converted into tetracycline hydrochloride /TC.HCl/.     

Recycling of NADP+ using immobilizedE. coli and glucose-6-phosphate dehydrogenase

Recycling of NADP⁺ using immobilized wholeEscherichia coli cells as source of respiratory chain, glucose-6-phosphate, and soluble yeast glucose-6-phosphate dehydrogenase (1.1.1.49) is described. NADP⁺ was recycled more than 10-fold. We demonstrated NADPH respiration at pH 5.8 inE. coli membrane vesicles. The respiratory chain was involved most probably in NADPH oxidation.

1. The respiratory activity is localized at the level of the inner bacterial membrane. The active site for NADPH facing the cytoplasm.
2. NADPH respiration is inhibited by 10 mM cyanide, similar to the conditions of inhibition of NADH respiration.
3. NADPH dehydrogenase activity seems to be the limiting step of the respiratory chain:K _M for NADPH respiration and NADPH dehydrogenase activity are similar. The pH optima for these two activities are also comparable (around pH 5.8). Furthermore, the following properties are rather in favor of a common NADH dehydrogenase and NADPH dehydrogenase activity (1.6.99.2).

o| li](1)|At saturating concentrations of NADH and NADPH, neither respiration nor dehydrogenase activities were additive. li](2)|Similar heat inactivation kinetics were observed for NADH and NADPH dehydrogenase-activity. Protection against heat inactivation was obtained for the two activities with NAD⁺, NADP⁺, NADH, and NADPH. All these results suggested the possibility of recycling of NADP⁺ under similar conditions to those previously described for NAD⁺ (Burstein et al., 1981). It becomes thus possible to use various NAD⁺ and NADP⁺-dependent dehydrogenases in enzyme technology.     

Gel-assisted synthesis of anatase TiO2 nanoparticles and application for electrochemical determination of L-tryptophan

Anatase titanium dioxide nanoparticles (TiO₂-NPs) were synthesized with and without gelatin via the sol-gel method. The TiO₂-NPs were characterized by a number of techniques, such as thermogravimetric analysis (TGA), X-ray diffraction analysis (XRD), transmission electron microscopy (TEM), fourier transform infrared spectroscopy (FT-IR) and ultraviolet visible spectroscopy (UV-Vis). The particle sizes of the TiO₂-NPs prepared with and without gelatin were ～13 and ～17 nm, respectively. The main advantage of using gelatin as a stabilizing agent is that it provides long-term stability for nanoparticles by preventing particles agglomeration. The results indicated that gelatin was a reliable green stabilizer, which can be used as a polymerization agent in the sol-gel method for synthesis of tiny size TiO₂-NPs. Moreover, the composite film was prepared by synthesized TiO₂-NPs nanoparticles and multi wall carbon nanotube (MWNT) on glassy carbon electrode (TiO₂-MWNT/GCE). The TiO₂-MWNT/GCE responded linearly to L-tryptophan (L-Trp) in the concentration of 1.0 × 10^?6 to 1.5 × 10^?4 M with detection limit of 5.2 × 10^?7 M at 3 using amperometry. The studied sensor exhibited good reproducibility and long-term stability.     

Ion beam irradiation of ZnS dispersed in PMMA and its photocatalytic application

ZnS nanoparticles implanted with 45 keV O⁵⁺ ion beam exhibited 83.6 % degradation of methyl blue in 2 h. This idea was utilized to fabricate nanocomposite system of ZnS and PMMA where ZnS nanoparticles were immobilized in PMMA film and irradiated with 45 keV O⁵⁺ ion beam at particle fluence of 2.5 × 10¹⁵, 1 × 10¹⁶ and 4 × 10¹⁶ particles/cm². These irradiated batches of ZnS nanoparticle immobilized in PMMA batches revealed formation of porous structure characterized by scanning electron microscopy and these batches exhibited 54 % photocatalytic degradation of methyl blue in 80 min which was higher as compared to the pristine ZnS nanoparticles.     

Flavin-protein interaction in bound glucose oxidase

Glucose oxidase was bound to Sepharose, Sephadex, gelatin, and dextran, yielding immobilized soluble and insoluble derivatives of the enzyme. The soluble preparations possessed higher enzymic activity than the analogous insoluble ones. The reversible dissociation process of the bound enzyme into apoenzyme and flavin adenine dinucleotide (FAD) was studied with the soluble and insoluble glucose oxidase in relation to enzymic activity and conformational changes as measured by circular dichroism and fluorescence methods. Bound apoenzyme was found to be more stable than the apoenzyme obtained from the unmodified glucose oxidase. The binding constant of FAD in bound glucose oxidase (K_diss≈10^-8M) calculated from fluorescent studies was lower than that of FAD in the native enzyme (K_diss10^-10M). The circular dichroism measurements indicated that dextran-bound glucose oxidase has a conformation similar to that of the native enzyme.     

Feasibility of in-house sterilization of laboratory plastic consumables using 2 MeV electron beam facility

In-house sterilization by electron beam (EB) radiation of various plastic consumables (plastic petridishes, micro centrifugal tubes and screw-capped vials) used routinely in the lab was studied by use of three microbiological cultures (S. aureus, Bacillus subtilis and Candida albicans). Current international standards (ISO 11137-Part 2 -ISO, 2011) recommend an irradiation dose of 25 kGy as a reference dose for terminal sterilization. All containers were exposed in an ILU-6, 2 MeV, 20 kW, Pulse EB accelerator located in our complex. Sterility test (S.T.) was performed and results revealed that 10⁶ and 10⁷ population of all strains passed whereas 10⁸ population failed S.T. for all micro-organisms indicating the potential of 2 MeV EB for commercial sterilization of plastic lab consumables for up to 10⁷ population of these micro-organisms.     

A sensor based on incorporating Ni2+ into ZnO nanoparticles-multi wall carbon nanotubes-poly methyl metacrylat nanocomposite film modified carbon paste electrode for determination of carbohydrates

The ZnO nanoparticles (ZnONPs) were synthesized with gelatin as stabilizer via the sol-gel method and were characterized by transmission electron microscope (TEM), scanning electron microscopy (SEM) and X-ray diffraction (XRD). An electrochemical sensor based on ZnO nanoparticles-multi wall carbon nanotubes-poly methyl metacrylat (ZnONPs-MWCNT-PMMA) composite film was developed by incorporating Ni²⁺ into the ZnONPs-MWCNT-PMMA film modified carbon paste electrode (Ni²⁺/ZnONPs-MWCNT-PMMA/CPE). The electrochemical activity of Ni²⁺/ZnONPs-MWCNT-PMMA/CPE was illustrated in 0.10 M NaOH using cyclic voltammetry. The Ni²⁺/ZnONPs-MWCNT-PMMA/CPE exhibits the characteristic of improved reversibility and enhanced current responses of the Ni(III)/Ni(II) couple. Ni²⁺/ZnONPs-MWCNT-PMMA/CPE also show good electrocatalytic activity toward the oxidation of carbohydrates (glucose, fructose and sorbitol). The Ni²⁺/ZnONPs-MWCNT-PMMA/CPE gives a good linear range with a detection limit of 8, 6, and 9 μM towards the determination of glucose, fructose and sorbitol, respectively by amperometry. Furthermore, the modified sensor was successfully applied to the sensitive determination of carbohydrates in real samples.     

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.     

On the determination of HCl+ (A,v′) vibrational populations from HCl+ (A→X) fluorescence spectra: direct comparison between photoionization and penning ionization

Using a beam apparatus, we have measured the HCl⁺ (A,v′→X,v″) fluorescence spectra of HCl⁺ (A,v′) ions formed in HeI (58.4 nm), and NeI (73.6 nm) photoionization and, for the first time, in He (2³ S) Penning ionization under single collision conditions with a wavelength bandwidth around 1 nm. In addition, we have studied Ne (3s ³ P _{2, 0}) Penning ionization of HCl at three different collision energies. The procedure and the problems in extracting HCl⁺ (A,v′) vibrational populations from the data are discussed in some detail. Thedirect comparison of photoionization and Penning ionization data allows definitive conclusions to be drawn on the question whether final state interactions in the Penning reaction change the “nascent” vibrational population (determined by electron spectrometry); for He (2³ S)+HCl, such changes are shown to be absent within the experimental uncertainty (<±10%). For Ne (3s ³ P _{2, 0})+HCl, the HCl⁺ (A,v′=0, 1) populations are also found to be close to those measured by electron spectrometry and essentially independent of collision energy in the range 34–96 meV. From measurements of the fluorescence intensity as a function of HCl density, we have evidence for a fast loss of HCl⁺ (A,v′) ions in collisions with HCl (rate constant around 5·10^?9 cm³s^?1).     

Purification of nerve growth factor from the venom of the Central Asian cobraNaja oxiana

A highly purified electrophoreticaly homogeneous protein with a NGF activity of 10·10⁵ BU/mg of protein have been isolated from the venom of the Central Asian cobra by gel-filtration and ion-exchange chromatography followed by preparative isolectric focusing in a thin layer of Sephadex. It has been shown that the NGF isolated is characterized by a molecular weight in the range of 20–30 kD and a pI value of about 7.0.     

Studies on the use of Sepharose-N-Aminohexanoyl-Glucosamine for purification of rabbit red blood cell hexokinase

N-acetyl glucosamine is a competitive inhibitor (K _t= 0.7 mM) of red blood cell hexokinase with respect to glucose. This property has been utilized for the purification of hexokinase by means of Sepharose-TV-aminohexanoyl-glucosamine. Studies with this matrix have proved that ionic strength and pH play a very important role in the binding of hexokinase to the affinity column. Therefore their control is essential in order to minimize nonspecific binding and to maximize the purification. Methods for rejuvenation of columns, the effect of protein concentration, and the nature of the binding are also discussed in this paper.     

Properties of human parotid amylase immobilized by covalent binding to glass or sepharose or by reaction with immobilized antibody

Human parotid amylase was immobilized by covalent binding to CNBr-activated Sepharose, to Corning GAO-3940 silica glass biomaterial support by the diazonium reaction or reaction with glutaraldehyde, or as a result of the antigen-antibody reaction between rabbit antihuman parotid amylase IgG that was covalently bonded to GAO glass and soluble amylase. The amylase directly bonded to the supports showed constant activity at flow rates of 3-15 ml/min through a 1.76-cm³ (8-mm diameter) support bed, did not lose enzyme into a circulating starch solution, retained its activity in the presence of soluble antiamylase IgG, was optimally active at 35°-40°C, and lost activity at 40°-45°C. When the enzyme was bound by interaction with immobilized antibody, full activity was expressed, but some enzyme was solubilized by a circulating starch solution. Immobilization of either amylase or antiamylase IgG makes dissolution of the antigen-antibody bond difficult.     

Immunomodulatory Response of Mice Splenocytes Induced by RcaL, a Lectin Isolated from Cobia Fish (Rachycentron canadum) Serum

This work reports the isolation of a serum lectin from cobia fish (Rachycentron canadum) named RcaL. Immunomodulatory activity on mice splenocyte experimental cultures through cytotoxic assays and cytokine production were also performed. RcaL was obtained through precipitation with ammonium sulphate and affinity chromatography on a Concanavalin A-Sepharose 4B column. The ammonium sulphate fraction F3 showed the highest specific hemagglutinating activity and was applied to affinity chromatography. The lectin was eluted with methyl-α-d-mannopyranoside. RcaL showed highest affinity for methyl-α-d-mannopyranoside and d-mannose; eluted fractions of RcaL agglutinated rabbit erythrocytes (titre, 128^?1) retained 66 % of chromatographed lectin activity, and the obtained purification factor was 1.14. Under reducing conditions, a polypeptide band of 19.2 kDa was revealed in sodium dodecyl sulphate polyacrylamide gel electrophoresis (PAGE). PAGE confirmed RcaL as an acidic protein revealed in a single band. Cytotoxic and immunomodulatory assays with RcaL in mice splenocyte cultures showed that the lectin was not cytotoxic and induced higher interferon gamma and nitric oxide production in splenocyte cultures. Purified RcaL induced preferential Th1 response, suggesting that it acts as an immunomodulatory compound.     

Synthesis of 5-phenyl-3-(10H-phenothiazinyl)-Δ2-cyclohexen-1-ones by conventional and microwave-assisted methods and their antifungal activity

A series of 5-phenyl-3-(10H-phenothiazinyl)-Δ²-cyclohexen-1-ones were prepared using conventional and microwave-assisted methods. The condensation between 3-phenyl-1-(10H-phenothiazinyl) prop-2-en-1-one derivatives (3a–g) and acetyl acetone yielded 5-phenyl-3-(10H-phenothiazinyl)-Δ²-cyclohexen-1-one derivatives (7a–g). The products were characterized by UV, IR, ¹H NMR, ¹³C NMR, 2D-NMR, MS, and elemental analysis. In vitro antifungal activity was carried out by zone of inhibition method against four species, namely Aspergillus niger, Candida albicans, Microsporum gypseum, and Aspergillus flavus. Compounds 7a and 7d showed good antifungal activity with zones of inhibition of 17 and 18 mm, respectively, and comparable with the standard substance, Bavinston, with 20 mm.