Estimation of the pK a of the amine groups of benzhydrylamine resin and its lysyl derivative by measurement of swelling

Summary For better evaluation of the potential of benzhydrylamine resin (BHAR), used as a solid support for peptide synthesis, as a novel anion-exchange resin, the pK _a of its amine group was estimated by microscopic measurement of the sizes of the dry and swollen beads. Using the volume of the bead occupied by the solvent (as a percentage) as the swelling parameter, a plot of the degree of swelling of BHAR loaded with 2.4 mmol g^–1 amine groups against the pH of the medium produced a decreasing sigmoidal-type curve with increasing pH. By considering the point of inflection of the curve, a pK _a value of approximately 7.5 was estimated for the amine group of the BHAR. The same approach was also applied to the lysyl derivative of the BHAR (Lys-BHAR) and pK _a values around 6.5 and 10.0 were obtained for the and amine groups, respectively.     

Poly(1-allylimidazole)-grafted silica,a new specific stationary phase for reversed-phase and anion-exchange liquid chromatography

A new specific stationary phase based on poly(1-allylimidazole)-grafted silica has been synthesized and characterized, by infrared spectra, elemental analysis, thermogravimetric analysis and X-ray photoelectron spectroscopy. The results of test showed that poly(1-allylimidazole) can effectively mask the residual silanol groups and reduce the adverse effect of residual silanol. Using this stationary phase, phenol compounds, aniline compounds, and polycyclic aromatic hydrocarbons were successfully separated with symmetric peak shapes in the reversed-phase chromatography. Inorganic anions (IO₃⁻, BrO₃⁻, Br⁻, NO₃⁻, I⁻, SCN⁻) were also separated completely in the anion-exchange chromatography using sodium chloride solution as the mobile phase. The effects of pH and the concentration of eluent on the separation of inorganic anions were studied. The separation mechanism appears to involve the mixed interactions of hydrogen bonding, hydrophobic, π–π, electrostatic, and anion-exchange interactions.     

Membrane chromatography: Protein purification from E. coli lysate using newly designed and commercial anion-exchange stationary phases

This contribution describes the purification of anthrax protective antigen (PA) protein from Escherichia coli lysate using bind-and-elute chromatography with newly designed weak anion-exchange membranes. Protein separation performance of the new AEX membrane adsorber was compared with the commercial Sartobind^® D membrane adsorber and HiTrap™ DEAE FF resin column under preparative scale conditions. Dynamic protein binding capacities of all three stationary phases were determined using breakthrough curve analysis. The AEX membrane showed higher binding capacities than the Sartobind^® D membrane at equivalent volumetric throughput and higher capacities than the HiTrap™ DEAE FF resin column at 15 times higher volumetric throughput. Anion-exchange chromatography was performed using all three stationary phases to purify PA protein. Quantitative SDS-PAGE analysis of effluent fractions showed that the purity of PA protein was higher for membrane adsorbers than the HiTrap™ DEAE FF resin column and was the same for the new AEX membrane and Sartobind^® D membrane adsorbers. The effects of E. coli lysate load volume and volumetric flow rate on PA protein separation resolution using the membrane adsorbers were minor, and the peak elution profile remained un-changed even under conditions where >75% of the total protein dynamic binding capacity of the membranes had been utilized. PA protein peak resolution was higher using pH-gradient elution than with ionic strength gradient elution. Overall, the results clearly demonstrate that membrane chromatography is a high-capacity, high-throughput, high-resolution separation technique, and that resolution in membrane chromatography can be higher than resin column chromatography under preparative conditions and at much higher volumetric throughput.     

Analysis of carbohydrates using different quaternized polystyrene-divinylbenzene particles and pulsed amperometric detection

Summary This paper reports on the use of a polymer-based, strong anion-exchange stationary phase for rapid, selective and sensitive analysis of physiological important mono-, di- and oligosaccharides by high-performance anion-exchange chromatography (HPAEC) with pulsed amperometric detection (PAD) under alkaline conditions. The adsorbent was obtained by direct nitration of 3 and 5 μm, spherical non-porous highly cross-linked, styrene-divinylbenzene copolymer (PS-DVB) beads, followed by reduction of superficially introduced nitro groups with nascent hydrogen and quaternization of the resultant amino groups with iodomethane. Extended exposure to high pressure and strong alkaline conditions did not have any untoward effect on mechanical stability and chromatographic performance. A comparison of the 3 and 5 μm beads showed, that the synthesized 3 μm highly cross-linked PS-DVB particles are the preferred phases for the separation of monosaccharides and the 5 μm particles are preferable for the separation of oligosaccharides. To demonstrate the suitability for the analysis of complex samples, the optimized and validated system was used for the determination of glucose, fructose and sucrose in apple juice and other soft drinks such as Coca Cola. Finally, analysis within a few minutes without sample pretreatment down to a lower limit of detection of 0.174–0.504 μg mL⁻¹ at a linearity with R²>0.994 and a repooducibility higher than 98% further confirmed the efficiency of these polymeric sorbents.     

The separation of synthetic mixtures of glucose and fructose and also inverted sucrose feedstocks using countercurrent chromatographic techniques

Summary A pilot scale semi-continuous countercurrent chromatographic Refiner (SCCR4) unit packed with a Zerolit 225 resin in the Ca²⁺ form has been used to separate synthetic mixtures of glucose and fructose and also inverted sucrose feedstocks into glucose-rich and fructose-rich products.For the same process conditions less pure fructose-rich products were found when using inverted sucrose feedstocks than with synthetic mixtures of glucose and fructose. However, anion-exchange resins Duolite A113 in the (HSO ₃ ^– ) form did not produce any variation in product purities with change of feed source.     

高效阴离子交换-脉冲安培检测同时分析单糖和糖醛酸

建立了高效阴离子交换-脉冲安培检测(HPAE-PAD)同时分离测定8种单糖和2种糖醛酸的分析方法。以CarboPacPA20阴离子交换柱为分离柱,以2mmol/LNaOH溶液将8种单糖从分离柱上洗脱,而后用NaAc(50~200mmol/L)梯度淋洗2种糖醛酸,淋洗液流速为0.5mL/min,总分析时间为30min。在优化的分离测定条件下,8种单糖和2种糖醛酸的检出限为2.5~14.4μg/L(进样体积25μL,峰面积定量)。5mg/L的10种化合物的混合标准溶液连续7次进样,峰面积的相对标准偏差为0.3%~1.5%。用所建立的方法测定了多糖水解液和木材半纤维素水解液中的单糖和糖醛酸含量。     

Liquid chromatography-hydride generation-atomic fluorescence spectrometry hybridation for antimony speciation in environmental samples

Atomic fluorescence spectrometry was used as an element-specific detector in hybridation with liquid chromatography (LC) and hydride generation for the speciation of Sb(III), Sb(V) and trimethylantimony dichloride (TMSbCl₂). The three species were poorly resolved in a single chromatogram but good results were obtained by anion-exchange chromatography, using a mobile phase with 20 mM EDTA and 8 mM hydrogenphthalate to separate Sb(III) and Sb(V) and 1 mM carbonate at pH 10 to separate Sb(V) and TMSbCl₂. Calibration graphs were linear between 2 and 100 μg l⁻¹. Detection limits were 0.9, 0.5 and 0.7 μg l⁻¹ for Sb(III), Sb(V) and TMSbCl₂, respectively. The method was applied to the speciation of antimony in environmental samples.     

Use of potassium-form cation-exchange resin as a conductimetric enhancer in ion-exclusion chromatography of aliphatic carboxylic acids

In this study, a cation-exchange resin (CEX) of the K⁺-form, i.e., an enhancer resin, is used as a postcolumn conductimetric enhancer in the ion-exclusion chromatography of aliphatic carboxylic acids. The enhancer resin is filled in the switching valve of an ion chromatograph; this valve is usually used as a suppressor valve in ion-exchange chromatography. An aliphatic carboxylic acid (e.g., CH₃COOH) separated by a weakly acidic CEX column of the H⁺-form converts into that of the K⁺-form (e.g., CH₃COOK) by passing through the enhancer resin. In contrast, the background conductivity decreases because a strong acid (e.g., HNO₃) with a higher conductimetric response in an eluent converts into a salt (e.g., KNO₃) with a lower conductimetric response. Since the pH of the eluent containing the resin enhancer increases from 3.27 to 5.85, the enhancer accelerates the dissociations of analyte acids. Consequently, peak heights and peak areas of aliphatic carboxylic acids (e.g., acetic acid, propionic acid, butyric acid, and valeric acid) with the enhancer resin are 6.3-8.0 times higher and 7.2-9.2 times larger, respectively, than those without the enhancer resin. Calibrations of peak areas for injected analytes are linear in the concentration range of 0.01-1.0 mM. The detection limits (signal-to-noise ratio = 3) range from 0.10 μM to 0.39 μM in this system, as opposed to those in the range of 0.24-7.1 μM in the separation column alone. The developed system is successfully applied to the determination of aliphatic carboxylic acids in a chicken droppings sample.     

Adsorption of Nb,Ta and Pa on anion-exchanger in HF and HF/HNO<Subscript>3</Subscript> solutions: Model experiments for the chemical study of Db

Anion-exchange behavior of the group-5 elements, Nb and Ta, and their pseudo homologue Pa in HF and HF/HNO₃ solutions was investigated by a batch method to find suitable conditions for the anion-exchange experiment of element 105 (Dubnium, Db). We determined the distribution coefficients of those elements on the anion-exchange resin as a function of the F⁻ and NO₃⁻ concentrations. Clearly different anion-exchange behavior was observed among these elements. Based on the results, we discuss the fluoro-complex formation of each element and suggest experimental conditions for the study of fluoride complexation of Db.     

强碱阴离子交换树脂及碱性洗脱剂的离子排阻/阴离子交换色谱法同时测定NH4+ ，NO2-和NO3-（英文）

Ion-exclusion/anion-exchange chromatography(IEC/AEC) on a combination of a strongly basic anion-exchange resin in the OH——form with basic eluent has been developed.The separation mechanism is based on the ion-exclusion/penetration effect for cations and the anion-exchange effect for anions to anion-exchange resin phase.This system is useful for simultaneous separation and determination of ammonium ion(NH+4),nitrite ion(NO-2),and nitrate ion(NO-3) in water samples.The resolution of analyte ions can be manipulated by changing the concentration of base in eluent on a polystyrene-divinylbenzene based strongly basic anion-exchange resin column.In this study,several separation columns,which consisted of different particle sizes,different functional groups and different anion-exchange capacities,were compared.As the results,the separation column with the smaller anion-exchange capacity(TSKgel Super IC-Anion) showed well-resolved separation of cations and anions.In the optimization of the basic eluent,lithium hydroxide(LiOH) was used as the eluent and the optimal concentration was concluded to be 2 mmol/L,considering the resolution of analyte ions and the whole retention times.In the optimal conditions,the relative standard deviations of the peak areas and the retention times of NH+4,NO-2,and NO-3 ranged 1.28%-3.57% and 0.54%-1.55%,respectively.The limits of detection at signal-to-noise of 3 were 4.10 μmol/L for NH+4,1.87 μmol/L for NO-2 and 2.83 μmol/L for NO-3.     

Ion-exclusion chromatography with the direct UV detection of non-absorbing inorganic cations using an anion-exchange conversion column in the iodide-form

An ion-exclusion chromatographic method for the direct UV detection of non-absorbing inorganic cations such as sodium (Na⁺), ammonium (NH₄⁺) and hydrazine (N₂H₅⁺) ions was developed by connecting an anion-exchange column in the I⁻-form after the separation column. For example, NH₄⁺ is converted to a UV-absorbing molecule, NH₄I, by the anion-exchange column in the I⁻-form after the ion-exclusion separation on anion-exchange column in the OH⁻-form with water eluent. As a result, the direct UV detection of Na⁺, NH₄⁺ and N₂H₅⁺ could be successfully obtained as well as the well-resolved separation. The calibration graphs of the analyte cations detected with UV at 230 nm were linear in the range of 0.001-5.0 mM. The detection limits at S/N = 3 of the cations were below 0.1 μM. This method was applied to real water analysis, the determination of NH₄⁺ in river and rain waters, or that of N₂H₅⁺ in boiler water, with the satisfactory results. This could be applied also to low- or non-absorbing anions such as fluoride or hydrogencarbonate ions by the combination of a weakly acidic cation-exchange resin in the H⁺-form as the separation column and the anion-exchange conversion column.     

Peak parking technique for the simultaneous determination of anions and cations

An ion chromatography method is described for the simultaneous determination of anions (Cl^–, NO₃^–, and SO₄^2–) and cations (Na⁺, NH₄⁺, K⁺, Mg²⁺, and Ca²⁺) using a single pump, a single eluent and a single detector. An anion-exchange column modified with chondroitin sulfate C facilitated the elution of the above three anions using 5 mM tartaric acid as the eluent in isocratic mode, whereas the same eluent facilitated the separation of the above five cations on a commercially-available cation-exchange column. The separation columns were connected in series via two six-port switching valves, so the required cation-exchange or anion-exchange separation could be carried out by selecting the appropriate positions for the switching valves. The separations were completed in 30 min.     

Observations on the effect of temperature on performance and stability of anion exchange columns in ion chromatography

Summary The influence of column temperature on elution behaviour of several ions on anion-exchange resin beds of the Dionex Ion Pac type was investigated. Iodate, bromate, bromide and iodide ions were separated on Ion Pac AS9SC column in the temperature range of 10°C–55°C, using NaHCO₃/Na₂CO₃ and NaHCO₃ eluents. Free energy, enthalpy and entropy changes for respective ion exchange reactions were calculated and compared with literature data for classical gel type exchangers. In most cases the enthalpy change was a function of temperature. The work at elevated temperatures caused progressing resin degradation i.e. loss of strongly basic groups, accompanied by formation of weakly basic groups and also some weakly acidic groups. Similar resin degradation was observed for Ion Pac AS5 column. Observations on the changes of the plate height with the retention factor and temperature lead to conclusion that in some circumstances longitudinal diffusion in the resin phase also contributes to the total plate height.     

Determination of Chlorophenols and Alkylphenols in Water and Juice by Solid Phase Derivative Extraction and Gas Chromatography–Mass Spectrometry

A solid phase derivative extraction method using acetic anhydride was developed for the determination of chlorophenols and alkylphenols in water and fruit juice by gas chromatography–mass spectrometry (GC–MS). The quantitative extraction was performed by passing 100 mL of sample prepared in 0.1 mol L^?1 sodium hydroxide through a column packed with 500 mg of a strong anion-exchange resin at a flow rate of 0.75 mL min^?1. The retained phenols were quantitatively derivatized in the column by the introduction of 0.25 mL of acetic anhydride. The derivatized phenols were eluted with 3.0 mL of hexane and the effluent was dried under nitrogen. The final volume was diluted to fifty microliters with hexane and analyzed by GC–MS. Under the optimum conditions, preconcentration factors of 2000, limits of detection between 0.005 and 1.796 µg L^?1, and relative standard deviations of 2.1% to 6.7% were obtained. The method was successfully applied to wastewater and fruit juice and the recoveries of phenols were between 76% and 111%.     

Radiochemical separation of 109Cd from a silver target

A radiochemical separation method was developed for the separation of ¹⁰⁹Cd from a ^nat.Ag target (6.6 g, pressed into a 19 mm disc). The method comprised of two stages. In the first stage, after dissolution of the target in nitric acid, silver was separated from Cd by precipitation into the metallic form using 20 g of Cu turnings for the reduction of Ag⁺ ions. In the second stage, ¹⁰⁹Cd in the filtrate, that contained trace amount of silver and substantial quantity of Cu(I), was purified by use of a Bio-Rad AG1-X10 anion-exchange resin. The ion-exchange chromatography employed a column with (1.6 cm i.d. and 4 cm length) with a flow rate of 2 ml/min throughout the separation. ¹⁰⁹Cd was quantitatively recovered from the first stage and the recovery yield from the ion-exchange chromatography was greater than 96%. 2M HCl containing H₂O₂ was used for the adsorption of ¹⁰⁹Cd and elution of Cu. ¹⁰⁹Cd was eluted by 50 ml 1M HNO₃. The concentrations of stable isotopes of Ag and Cu in the final solution (5 ml 0.05M HCl) were measured by an ICP-OES method and found to be <1 ppm.     

The stationary phase capacity concept in elution liquid chromatography

The stationary-phase capacity concepts derived from linear capacity are discussed in connection with the needs of analytical, trace enrichment analysis and preparative chromatography and shown to be unsuited to them. A new concept based on stationary-phase saturation and called “available capacity” is proposed. It generalizes the ion-exchanger exchange capacity to adsorption and partition chromatography when the sampling solvent is the mobile phase. In linear elution chromatography the available capacity is proportional to the solute concentration C_o and to the analytical capacity factor k′ for given C_o and k′ values, it is independent of the nature of the solute. Furthermore, when both the concentrations and the analytical capacity factors (practically, for C_o ≥ 1 M and k′ ≥ 10, respectively) are high, the available capacity reaches a value roughly independent of C_o and k′, called “maximum available capacity” and related only to the number of sites available on the stationary phase. Numerous measurements were made in ion-exchange, adsorption, and reversed-phase chromatography. For solutes having a single polar functional group interacting with the stationary phase, the orders of magnitude of the maximum available capacity are 1.2 mmole g^?1 for a classical silica gel (Partisil 5 μm, 400m^?2 g^?1 with a water content of 2.7%); 1.8 mmole g^?1 for the Lichroprep RP 8 octyl bonded silica (11.6% carbon content); 3.8 mmole g^?1 for an anion exchanger resin of Dowex type.     

Copper modified platinum electrode for amperometric detection of spectinomycin sulfate by anion-exchange chromatography

A La~(3+)-Cu/Pt modified electrode was fabricated by electrodepositing process in CuSO_4 solution by adding a small amount of lanthium compound,and it was employed for direct current(DC) amperometric detection of spectinomycin by anion-exchange chromatography.Without derivatization,this method can simultaneously determine the main component and impurities in spectinomycin pharmaceutical raw material.Ease of preparation,being applied in DC detection mode and good catalytic stability confirmed the interest...     

Simultaneous determination of oxalate, thiosulfate, and thiocyanate in urine by ion-exclusion chromatography with electrochemical detection

Summary A sensitive ion-exclusion chromatographic method has been developed for determination of oxalate, thiosulfate, and thiocyanate. The method is based on separation of these anions on a polymethacrylate-based, weakly acidic cation-exchange resin (TSKgel OApak-A) and detection by means of a glassy carbon (GC) electrode electrochemically modified with polyvinylpyridine (PVP), palladium, and iridium oxide (PVP/Pd/IrO₂). The electrochemical behavior of oxalate, thiosulfate, and thiocyanate at this chemically modified electrode (CME) have been investigated by cyclic voltammetry. The results indicated that electrocatalytic oxidation of these anions by the electrode was efficient and that the sensitivity, stability, and lifetime of the electrode were relatively high. Combined with ion-exclusion chromatography the PVP/Pd/IrO₂ electrode was used as the working electrode for amperometric detection of these anions. All linear ranges were over two orders of magnitude and detection limits, defined asS/N=3, were 9.0×10⁻⁷ mol L⁻¹ for oxalate, 6.7×10⁻⁷ mol L⁻¹ for thiosulfate, and 5.6×10⁻⁷ mol L⁻¹ for thiocyanate. Correlation coefficients were all>0.998. Coupled with microdialysis sampling the method has been successfully applied to the determination of oxalate, thiosulfate, and thiocyanate in urine.     

Preparation of strong anion-exchange chromatographic packings based on monodisperse polymeric beads and their application in the separation of biopolymers

A new hydrophilic strong anion-exchange (SAX) stationary phase for HPLC has been synthesized by chemical modification of macroporous 8.0-m monodisperse poly(glycidylmethacrylate-co-ethylenedimethacrylate) beads (P_GMA/EDMA). The stationary phase was evaluated in detail to determine its ion-exchange properties, separability, reproducibility, hydrophilicity, and the effect of column loading and pH on the separation and retention of proteins. It was found to have an ion-exchange chromatographic (IEC) retention mechanism. The highest dynamic protein loading capacity of the synthesized SAX packing for BSA was 22.6 mg g^–1. Five proteins were separated within 6.0 min using the synthesized SAX resin. The SAX resin was also used for rapid separation and purification of recombinant human stem cell factor (rhSCF) from a crude extract solution in only one step. The purity of the purified of rhSCF was >92.4%.     

高温热水解离子色谱法快速同时测定粘土中的卤素

建立高温热水解分解粘土样品,离子色谱快速同时测定其中的氟、氯、溴和碘含量的方法。优化了影响粘土高温热水解的主要参数,得到以下最佳测定条件:2.0 g粘土,反应温度1000℃,停留时间10 min,样品与催化剂V2O5质量比为1∶1,空气流量90 mL/min,15 mL 5.4 mmol/L Na2CO3和5.1 mmol/L NaHCO3混合溶液为粘土释放卤素的吸收液;考察了粘土高温热水解后卤素的赋存形态。结果表明,这些卤素在吸收液中以F!、Cl!、Br!和I!形式存在,且能被离子色谱很好地分离。粘土样品较好的卤素加标回收率和较小的相对标准偏差及土壤标准物质中卤素的评估说明本方法的准确度和精密度良好。分析了4个粘土样品,氟、氯、溴和碘的检出限分别为0.030,0.043,0.09和0.13#g/g,本方法简单、可靠、低消耗和快速,每小时可分析5个样品,可同时分析粘土和其它无机基质中的氟、氯、溴和碘的含量。