Isolation and purification oil glucuronides with preparative anion exchange chromatography in methanol

890 ml of urine of rats treated with [¹⁴C] 205–734 was desalted over an Amberlite XAD-2 adsorption column. The methanol extract dissolved in 10 ml methanol was injected onto an anion exchange column (Nucleosil 10 SB 250 × 16 mm i.d.) equilibrated in methanol. A gradient of decreasing methanol proportion versus a 0.2 M ammonium hydrogen carbonate buffer eluted a pure glucuronide of 205–734. Its structure was established by NMR, MS, UV, and IR analyses. This procedure is simple, rapid, and very selective for the compound of interest.     

Simultaneous anion and cation exchange chromatography of whey proteins using a customizable mixed matrix membrane

Membrane chromatography can overcome some of the limitations of packed bed column chromatography but preparation of adsorptive membranes usually involves complex and harsh chemical modifications. Mixed matrix membranes (MMMs) require only the physical incorporation of an ion exchange resin into the membrane polymer solution prior to membrane casting. An advantage of MMMs not previously exploited is that resins with differing adsorptive functionalities can be conveniently embedded within a single membrane at any desired ratio. This presents the opportunity to customize an adsorptive membrane to suit the expected protein profile of a raw feed stream e.g. bovine whey or serum. In this work, a novel mixed mode interaction MMM customized to extract all major proteins from bovine whey was synthesized in a single membrane by incorporating 42.5 wt% Lewatit MP500 anionic resin and 7.5 wt% SP Sepharose cationic resin into an ethylene vinyl alcohol base polymer casting solution. The mixed mode MMM developed was able to bind both basic and acidic proteins simultaneously from whey, with binding capacities of 7.16±2.24 mg α-lactalbumin g(-1) membrane, 11.40±0.73 mg lactoferrin (LF)g(-1) membrane, 59.21±9.90 mg β-lactoglobulin g(-1) membrane and 6.79±1.11 mg immunoglobulin Gg(-1) membrane (85 mg total protein g(-1) membrane) during batch fractionation of LF-spiked whey. A 1000 m(2) spiral-wound membrane module (200 L membrane volume, 1m(3) module volume) is predicted to be able to produce approximately 25 kg total whey protein per h.     

Direct preparative resolution of racemic amino-acids using ligand exchange chromatography (chirallec)

Summary Preparative resolutions of racemic amino-acids by ligand-exchange chromatography are described. Base-line resolution of multigram quantities of many racemic solutes was obtained using very simple equipment (open tubular column).     

Computer simulation of non-linear preparative chromatography processes

Summary A theory of non-linear chromatography based on the mass balance equation is presented. The model is a system of partial differential equations and it includes axial dispersion in the mobile phase, flow in the mobile phase and mass transfer between phases. In the case of the injection of a mixture competition between components for places in the stationary or the mobile phase is taken into account. In the paper are discussed: numerical calculations of concentration and volume overloading and the effect of the mutual influence of the components of the injected mixture on the process of mass transfer between phases. Additionally, results of experiments for convex and concave adsorption isotherms are presented. In both cases the results obtained qualitatively confirm the theoretical analyses.     

Separation of alkylnaphthalenes by preparative liquid chromatography using column switching systems

Summary The paper describes the separation of the mixture of alkynaphthalenes from distillation cuts of a pyrolysis oil, by preparative liquid chromatography on silica. The design of the system permits the connection of the columns to form multicolumn systems.The samples were first separated on a single column. The mixtures were further separated using two-column chromatography systems.The obtained fractions were analyzed by capillary gas chromatography. In most cases a substantial increase in the concentrations of the individual components was achieved. In several cases, pure compounds have been obtained. Separation efficiency increases in the following order: single column, two directly coupled collumns, two-step switching chromatography, heartcutting.     

Separation of ortho-substituted tetraphenylporphyrins by preparative HPLC

Summary A method for the separation of substituted tetraphenylporphyrins by preparative liquid chromatography is reported. The quality of the columns formed by axial compression of various stationary phases is tested.     

High performance displacement chromatography of proteins: Separation of β-Lactoglobulins A and B

Summary β-Lactoglobulins A and B were separated by high performance displacement chromatography on an anion-exchanger column with chondroitin sulfate as the displacer. A sample of 100 mg containing a mixture of the two β-lactoglublins was separated on a column of 75×7.5 mm in a single chromatographic run. The separation process followed the rules of the classical displacement development: the two proteins formed contiguous rectangular bands and their concentrations were dependent on the displacer concentration. The results demonstrate that high performance displacement chromatography is a useful technique for the separation of proteins in preparative amounts with columns and instrumentation typically used in analytical HPLC. Furthermore, it has the potential to become the method of choice in large scale separation of proteins.     

Application of a new capsule-type silica gel coated with hydrophobic polymer to preparative liquid chromatography on an industrial scale

Summary A new type of column packing material designed for preparative liquid chromatography, silicone polymer-coated silica gel modified with octadecyl group (S/S-C₁₈), was applied to chromatographic purification of a lipophilic biotechnological product. Triglycerides containing γ-linolenic acid were separated from the curde oil that consisted of triglycerides, diglycerides, free fatty acids, sterols and other polar substances, using a S/S-C₁₈ packed column (150 mm I.D. × 1000 mm). No column deterioration was observed after more than 1500 times of sample introductions.     

Separation of epigallocatechin and flavonoids from Hypericum perforatum L. by high-speed counter-current chromatography and preparative high-performance liquid chromatography

High-speed counter-current chromatography (HSCCC) and preparative high-performance liquid chromatography (prep-HPLC) were successively used for the separation of epigallocatechin and flavonoids from Hypericum perforatum L. The two-phase solvent system composed of ethyl acetate–methanol–water (10:1:10, v/v) was used for HSCCC. About 900 mg of the crude extract was separated by HSCCC, yielding 7.8 mg of quercitrin at a purity of over 97%, 12.6 mg of quercetin at a purity of over 93%, and 38.9 mg of a mixture of hyperoside, isoquercitrin and miquelianin constituting over 97% of the fraction. A mixture of epigallocatechin and avicularin pooled from three HSCCC runs, a total amount of 54.3 mg, was further separated by prep-HPLC yielding 23.4 mg of epigallocatechin and 15.3 mg of avicularin each at a purity of over 97%.     

Purification of thymine dimer from monomer solution in preparative liquid chromatography

Summary Cyclobutane pyrimidine dimers and monomers of thymine were separated on a C₁₈ reversed-phase high performance liquid chromatographic column. Using two mathematical models, the effect of the sample sizes on peak shapes in preparative liquid chromatography was investigated. One of these approaches is through a linear kinetic model, and the other is based on the non-linear adsorption isotherm. With the injection of small samples good agreement between the calculated value by the linear kinetic model and experimental, data were achieved. With increased sample size, this model is defective in its prediction of large concentration profiles of sample. However, the nonlinear model permits the accurate prediction of the location of the component band and the determination of the appropriate time to start and stop collection of the enriched fraction at higher concentrations of monomer and the lower concentrations of dimer. Therefore, extremely small amounts of dimer can be extracted from monomer solutions.     

A simplex optimization of the experimental parameters in preparative liquid chromatography

Summary A study of the optimization of the experimental conditions for the purification or extraction of pure compounds by liquid chromatography is presented. Optimum values of the parameters of overloaded elution are derived for maximum production rate, using a Simplex algorithm and the procedure previously described for the simulation of the elution profiles of binary mixtures. The mobile phase flow velocity and the sample size have been optimized together in a first step, simulating the procedure followed in practice, when a column is available. In a second part, the influence of the column length and the average particle size of the packing material on the column performance as well as the trade-offs between the production rate and the yield are discussed.There are three major conclusions in this work. First, the optimum experimental conditions are often very different, depending whether one is primarily interested in the first or in the second eluted component of a mixture. Second, the column efficiency under analytical conditions is very important: it is traded-off for high flow rates, hence short cycle time and increased production rate. Third, the production rate depends strongly on the maximum pressure at which the equipment can be operated. Finally, the optimum production rate varies rather smoothly with the mobile phase velocity and the sample size, so a high yield (70% or more) can usually be obtained with a limited loss in production rate (30 to 60%).     

Mass overload in preparative liquid chromatography: Choice of column dimensions and optimum working conditions

Summary This paper deals with a theoretical study which makes it possible to calculate column dimensions (length and inner diameter) and to select working conditions (particle diameter of the column packing, elution flow rate, run number) with regard to purity, recovery ratio and amount of pure substance that is to be isolated. These determinations take into account the pressure limitation and pumping capacity of the available chromatograph.     

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.     

S-trityl-(R)-cysteine, a powerful chiral selector for the analytical and preparative ligand-exchange chromatography of amino acids

S-trityl-(R)-cysteine [(R)-STC] is the new selector of a dynamically coated, chiral ligand-exchange stationary phase which proved to be highly effective in both analytical and preparative-scale separation of enantiomers of some natural and unnatural underivatized amino acids, with good separation and resolution factors. With the aim of identifying the best chromatographic conditions suitable for the preparative-scale separations, some parameters controlling retention, separation and resolution factors (such as the type and amount of cupric salt and the eluent pH) were investigated. The relatively easy removal of the Cu(II) ions renders this technique suitable for obtaining small amounts of enantiomerically pure samples for preliminary biological evaluations.     

Preparative liquid chromatography: Choice of column dimensions and working conditions for occasional preparative separation

Summary This paper deals with a theoretical study which makes it possible to calculate column dimensions (length and inner diameter) and working conditions (particle diameter of the stationary phase, elution flow rate, run number) with regard to purity, recovery ratio and the amount of pure substance that may be isolated. This determination takes into account the pressure limitation and pumping capacity of the available chromatograph. The isolation of microgram amounts of a component is shown in order to illustrate the above-mentioned calculation method.Presented at the 14th International Symposium on Chromatography London, September, 1982     

超大孔离子交换制备色谱分离纯化高活性凝血因子VIII

建立了一条从人血浆中分离高活性凝血因子VIII(FVIII)的纯化工艺。基于FVIII和介质孔径的尺度比及其对蛋白质活性影响的分析,设计了以超大孔离子交换制备色谱为核心步骤的新型分离纯化工艺。分别进行超大孔离子交换色谱与传统离子交换色谱的条件优化,并对优化工艺所得产品进行了活性检测(底物显色法)和纯度检测(高效凝胶过滤和凝胶电泳)。结果表明,超大孔介质结构不但可以有效地保护蛋白质大分子结构,而且能够大幅度地提高制备色谱的传质速率,从而得到具有高凝血活性的FVIII产品。FVIII在超大孔制备色谱过程中的回收率(85%)比传统离子交换制备色谱高4～5倍,产品比活高达154 IU/mg。此外,还研究了超大孔介质的再生程序,采用5个柱体积的1 mol/L NaOH低流速清洗色谱柱,保证了色谱工艺的稳定性。本纯化工艺步骤简单,重现性好,易于放大生产。     

Practical method for the definition of chromatographic peak parameters in preparative liquid chromatography

A practical method was established for the definition of chromatographic parameters in preparative liquid chromatography. The parameters contained both the peak broadening level under different amounts of sample loading and the concentration distribution of the target compound in the elution. The parameters of the peak broadening level were defined and expressed as a matrix, which consisted of sample loading, the forward broadening and the backward broadening levels. The concentration distribution of the target compound was described by the heat map of the elution profile. The most suitable stationary phase should exhibit the narrower peak broadening and it was best to broaden to both sides to compare to the peak under analytical conditions. Besides, the concentration distribution of the target compounds should be focused on the middle of the elution. The guiding principles were validated by purification of amitriptyline from the mixture of desipramine and amitriptyline. On the selected column, when the content of the impurity desipramine was lower than 0.1%, the recovery of target compound was much higher than the other columns even when the sample loading was as high as 8.03 mg/cm³. The parameters and methods could be used for the evaluation and selection of stationary phases in preparative chromatography.     

Optimization of throughput in preparative column luquid chromatography by column overloading and partial fractionation of the effluent

Summary The criteria for the optimization of preparative chromatography are sample throughput and product purity. It is shown for column liquid chromatography that the throughput has been maximized for a given purity by column overloading and appropriate fractionation. The size and position of the fraction must be determined by chemical analysis, since overlapping peaks under overloading conditions are usually distorted compared to the peaks of the same amounts of pure compounds. With overloading of the column larger particles can be used as column packings without reduction of the separation effect.     

反相液相制备色谱法结合超临界流体制备色谱法分离纯化海风藤中的化合物

建立了基于反相液相制备色谱和超临界流体制备色谱的组合方法,用于分离纯化醇提水沉后石油醚层中的海风藤。首先以甲醇作为改性剂,采用醇提水沉法去除海风藤甲醇提取物中的叶绿素,加入硅藻土后用石油醚回流富集目标成分。选用反相C18制备色谱柱将其分为18个组分,然后将组分在SFC模式下进行制备。选用酰胺色谱柱,以甲醇为改性剂,在柱温30℃、背压15.0 MPa的条件下进行分离。基于反相色谱和超临界流体色谱不同的分离选择性,最后分离得到6个高纯度化合物。该法展示了反相制备色谱和超临界流体制备色谱在海风藤分离纯化方面的优势,特别是超临界流体色谱在天然产物的分析和制备方面的巨大潜力。