Antibody capture by mixed-mode chromatography: a comprehensive study from determination of optimal purification conditions to identification of contaminating host cell proteins

We evaluated mixed mode chromatography for the capture of recombinant antibodies from CHO cell culture supernatants. We studied PPA HyperCel, HEA HyperCel, MEP HyperCel and Capto adhere resins, which all contain hydrophobic and cationic groups. A microplate approach combined with DoE modeling allowed the exploration of the complex behaviors of these mixed mode resins. Optimal conditions for antibody purification and host cell proteins (HCPs) elimination were determined and then directly up-scaled to laboratory columns. Then we used mass spectrometry to identify the major HCPs potentially coeluted with the antibody. Differences between the four resins in terms of amount, complexity and identity of the HCPs present in the elution fractions were investigated.     

Optimization of working conditions for polyelectrolyte sorbents

Matters affecting the working stability of polyelectrolyte sorbents are considered. The decrease in retention time during exploitation is found not to relate to desorption of the modifying polymer. It is found that dissociation of surface silanol groups influences significantly the extra retention of ionene on the surface of silica-based sorbents. Sorption of heavy metals and microbial contamination of the sorbent are identified as causes of decreased efficiency of polyectrolyte sorbents. The influence of organic additives on the chromatography behavior of a number of inorganic anions is studied. Finally, exploitational conditions for chromatography polyelectrolyte-containing columns are elaborated, allowing the initial parameters of separation to be maintained for a period of 1.5 months or longer.     

Separation of 1,4-Dihydropyridine Derivative and Its Oxidized Form

Derivatives of 1,4-dihydropyridine (DHP) still play an important role in treatment of cardiovascular diseases. Typical degradation of the DHP ring is aromatization to pyridine ring which occurs both chemically and biochemically. It is, therefore, important to have a reliable and robust analytical method for separation of DHPs from their oxidized counterparts. Separation of closely-related substances possessing similar hydrophobicity, such as DHP and its oxidized form, can be challenging on conventional alkyl-bonded sorbents. In this study, an impact of reversed-phase (RP) liquid chromatography conditions on separation of the DHP/Ox pair has been investigated. Initially, a systematic study has been performed on 33 commercial RP columns with mobile phase acetonitrile/water for separation of foridone and its corresponding oxidized form. The retention and selectivity are discussed in view of the hydrophobic-subtraction model. Best separation was found replacing conventional C₁₈ sorbents with ones containing an embedded polar group due to polar interactions. Similarly, application of cyano columns resulted in efficient separation of analytes. Organic modifier of mobile phase (methanol vs. acetonitrile) contributed significantly to separation of foridone from its oxidized counterpart. Separation of six chemically diverse DHPs from corresponding oxidized forms was studied on seven RP columns (traditional C₁₈ sorbent, alkyl sorbent with polar embedded group, two different aromatic phases, pentafluorophenylpropyl sorbent and sorbent with straight chain perfluorohexyl ligand). Both acetonitrile and methanol were applied as organic modifier. It was found that application of alkyl sorbent with an embedded polar group (column Zorbax Bonus RP) or cyano sorbent (column ACE CN) yields clear separation of chemically diverse DHPs from their oxidized forms.     

Monolithic capillary columns based on pentaerythritol acrylates for molecular‐size‐based separations of synthetic polymers

Monolithic capillary columns based on pentaerythritol triacrylate and pentaerythritol tetraacrylate were synthesized using different compositions of polymerization mixtures and different polymerization conditions. The impact of porogen type and porogen/monomer ratio on the porosity of synthesized monoliths was investigated. Porogen type appears to be the main factor influencing the separating properties of the monolithic sorbent. Using optimal polymerization conditions (porogen type, porogen/monomer ratio, reaction temperature, time etc.) monoliths with a porous structure optimized for polymer separations can be obtained. The monolithic capillary columns containing porous sorbents with optimized porosity are capable of separating 10 to 12 polystyrene standards in one chromatographic run utilizing both size exclusion chromatography and hydrodynamic chromatography separation mechanisms.     

A new general approach to purify proteins from complex mixtures

The selection of chromatography media and their sequential use represent a major difficulty to isolate a single protein from very crude protein extracts. The process described here consists of two main steps: (i) a rational selection of few media from a relatively large collection and (ii) the definition of the sequence of columns to get the best purity of the target protein. From the first step, one sorbent is selected for its properties to capture the protein to purify, regardless whether other protein impurities are also co-adsorbed; then 5-7 other complementary sorbents are identified to remove impurities but without interacting with the target protein under the same buffering conditions. The second step consists in superimposing sorbents under a cascade manner with the sorbent in charge to capture the target protein located in the last position. Non-adsorbed proteins are eliminated in the flowthrough; other impurities are progressively removed by the sorbent sequence and the target protein is finally desorbed and isolated from the last sorbent using an optimized gradient. All operations are performed with a single adsorption buffer for all columns and all monitoring performed by means of mass spectrometry associated with ProteinChip arrays and polyacrylamide gel electrophoresis. Examples of protein isolation/identification from human serum are described namely thyroxin-binding proteins and transferrin. The first is isolated thanks to a series of dye chromatography media, the second (transferrin) using current chromatographic media. In both cases the target proteins were purified at a level estimated of about 95% and 85%, respectively. Isolated proteins were pure enough for the purpose of formal identification by either peptide fingerprinting or sequencing.     

Ligand exchange chromatography for analysis and preparative separation of tritium-labelled amino acids

Racemic tritium-labelled amino acids were separated into optical isomers by chromatography on a chiral polyacrylamide sorbent filled with copper ions. The polyacrylamide sorbent is synthesized by Mannich's reaction through the action of formaldehyde and L-phenylalanine upon polyacrylamide Biogel P-4 in an alkali phosphate buffer. Tritiumlabelled amino acids are eluted by a weak alkali solution of ammonium carbonate. Data are presented on the ligand exchange chromatography of amino acids depending on the degree to which the sorbent is filled with copper ions and on the eluent concentration. Conditions are suggested for the quantitative separation of amino acid racemates. Amino acids are isolated from the eluent on short columns filled with sulfonated cation exchanger in the H⁺ form. HPLC on modified silica gel sorbents is also used for the analysis of tritium-labelled optically active amino acids. Amino acids are eluted by a weakly acidic water-methanol solution containing ammonium acetate. UV and scintillation flow type detectors are used.     

Nanoporous carbon sorbent for molecular-sieve chromatography of lipoprotein complex

The physicochemical characteristics of carbon sorbents are investigated. Electron microscopy data for the sorbent and separated lipoprotein complex are presented. It is found that the obtained carbon sorbent possess high porosity. Nanoporous carbon sorbents for the chromatography of molecular-sieve markers are obtained and tested. The applicability of nanoporous carbon sorbents for separation of lipoprotein complexes (LPC) is investigated.     

Contributions of commercial sorbents to the selectivity in immobilized metal affinity chromatography with Cu(II)

Immobilized copper(II) affinity chromatography [Cu(II)-immobilized metal affinity chromatography (IMAC)] has been used in proteomics to simplify sample mixtures by selecting histidine-containing peptides from proteolytic digests. This paper examines the specificity of four different support materials with an iminodiacetic acid (IDA) stationary phase in the selection of only histidine-containing peptides in the single step capture-release mode. Three of the sorbents examined were commercially available: HiTrap Chelating HP (agarose), TSK Chelate-5PW, and Poros 20MC. IDA was also immobilized on CIM discs (monolithic glycidylmethacrylate-ethylene dimethacrylate). Tryptic digests of transferrin and beta-galactosidase were used as model samples to evaluate these sorbents. It was found that among the examined matrices, the TSK Chelate-5PW sorbent bound histidine-containing peptides the strongest, while Poros matrix was found to have a high degree of non-specific bindings. Agarose-based columns showed relatively high selectivity and specificity.     

Permeability, porosity, and structure of monolithic capillary columns in gas chromatography

The permeability of monolithic silica gel capillary columns with respect to the helium carrier gas was studied using gas chromatography. The results obtained by gas chromatography and liquid chromatography were found to be in close agreement. The permeability of monolithic capillary columns was compared to that of hollow capillary columns and columns packed with finely dispersed sorbents. It was demonstrated that the permeability of the monolithic capillary columns studied is almost three orders of magnitude lower than that of hollow capillary columns of the same diameter but two orders of magnitude higher than that of columns packed with micron-scale particles. The interstitial fraction of the monolithic columns was found to be very high, 0.95.     

A novel sorbent for the determination of clenbuterol in bovine liver.

The use of three C18 sorbents in matrix solid phase dispersion (MSPD) for the determination of clenbuterol in bovine liver fortified at 5 ng g-1 is described. MSPD grade C18 sorbents give rise to more efficient blending and packing of the material for subsequent washing and analyte elution in comparison with a non-MSPD grade C18 sorbent. Following enzymatic deconjugation of the liver extracts, radioimmunoassay is used as the method of determination. The mean recovery of clenbuterol with all sorbents is comparable and within the range 86-96% in two intra-assay studies (n = 3). The liver extracts in each case are highly coloured. The variation in recovery is observed to be lowest with MSPD grade C18 (end-capped). This sorbent was used in further studies to evaluate the use of solid phase extraction (SPE), post MSPD, with normal phase aminopropyl or mixed mode cation exchange columns for extract purification. The mean recovery of clenbuterol (n = 4, inter-assay study) following MSPD and normal phase SPE clean-up was 95 +/- 15% and 89 +/- 9% at fortification levels of 1 and 2.5 ng g-1, respectively.     

Sorbent material characterization using in‐tube extraction needles as inverse gas chromatography column

In‐tube extraction is a full automated enrichment technique that consists of a stainless‐steel needle, packed with sorbent material for the extraction of volatile and semivolatile compounds. In principle, all particulate sorbents used for enrichment in air or headspace analysis can be used. However, the selection of the sorbents is merely based on empirical considerations rather than on experimental data, which is caused by a lack of knowledge about the relevant physicochemical properties of the sorbent. Especially, the knowledge of hydrostatic, advective, diffusive, and dispersion mechanisms in addition to sorption enthalpies are important for combined transport and sorption models. To provide these missing parameters, we developed and evaluated a method in which an ordinary in‐tube extraction needle was employed directly as column for sorbent characterization by inverse gas chromatography. As probe compounds, benzene, ethyl acetate, and 3‐methyl‐1‐butanol were used to determine thermodynamic parameters such as sorption enthalpy, partitioning constant between the solid and gas phase, and kinetic parameters such as the diffusion coefficient, dispersion coefficient, and apparent permeability, exemplarily. As sorbent, three commercially available phases were characterized to demonstrate the applicability of the method.     

Removal of organic pollutants from aqueous solution. V. Comparative study of the extraction, recovery and chromatographic separation of some organic insecticides using unloaded polyurethane foam columns

The concentration of dissolved insecticides in aqueous media was determined by chromatographic separation on polyurethane foam columns. The results of preliminary screening tests on the removal of insecticides by the unloaded polyurethane foam indicated that a reasonable percentage of the insecticides was retained on the foam. Therefore attempts were made to extract these compounds from aqueous media using foam columns. Various parameters affecting the retention and separation of these compounds were studied, including temperature, flow-rate, pH, insecticide concentration, shaking time, sample volume and eluting solvent. The complete separation and quantitative recovery of these compounds from the foam with acetone in a Soxhlet extractor were achieved. The method can be used to preconcentrate insecticides in tap water and modified to determine dissolved insecticides in industrial and natural waters. Polyurethane foam has a good capacity for use when large volume samples need to be handled and is an inexpensive sorbent compared to other known solid sorbents.     

Hydrophobic interaction chromatography of proteins. I. Comparison of selectivity

Currently, the selection of a hydrophobic interaction chromatography (HIC) sorbent for protein separation purposes is entirely based on empirical means. An attempt was made to characterize different HIC sorbents from various manufacturers. The selectivity was determined by isocratic pulse experiments of a set of reference proteins and an algorithm was developed to classify the sorbents according to their selectivity and hydrophobicity. The obtained semi-quantitative parameters take into account the dependence of salt on adsorption. The sorbent characteristics evaluated with the model proteins were compared to the separation of a real feedstock. A good agreement was achieved between the developed evaluation procedure and the separation behaviour of the real feed stock.     

Review. Use of laser detectors in capillary liquid chromatography

The main relationship of high-performance liquid chromatography (HPLC) are considered. It is shown that the optimum conditions of ultrasensitive trace analysis should be achieved by using packed capillary columns manufactured from flexible quartz capillaries with dc approximately less than 0.2 mm. The main features of these columns (v opt = 0.6 v opt of that for conventional HPLC columns with double the hydraulic permeability) make it possible to obtain two or three times higher plate numbers for the same analysis time and column pressure characteristic of conventional HPLC, as a result of using a submicrometre sorbent. The main features of laser detection in capillary liquid chromatography (laser-induced fluorescence and cross-beam thermal lens absorption detectors) are considered. The requirements that should be met by a modern capillary liquid chromatograph based on using flexible quartz capillary columns with a submicrometre sorbent and laser detectors are formulated. Examples of using these systems for femtomole and attomole analyses of biological samples (amino acids and prostaglandins) are given.     

吸收增强式甲烷水蒸气重整制氢循环反应模拟

吸收增强式甲烷水蒸气重整制氢反应可以生成高浓度的H2和较低浓度的CO、CO2。研究建立了考虑钙基吸收剂活性下降对吸收增强式甲烷水蒸气重整制氢过程影响的多次循环反应模型,在实验数据验证的基础上,计算了三种吸收剂活性下降特性对吸收增强式重整制氢过程的影响。结果表明,对于石灰石吸收剂,产生高纯H2的时间随循环次数的增加而急剧下降;白云石循环反应活性提高,产生高纯H2的时间随循环次数的增加而缓慢下降;CaO/Ca12Al14O33的循环使用次数明显大于石灰石和白云石。     

Extraction of biogenic amines using sorbent materials containing immobilized crown ethers

Three sorbent materials (A18C6-MS, DA18C6-MS and AB18C6-MS) based on the crown ether ligands, 1-aza-18-crown-6, 1,4,10,13-tetraoxa-7,16-diazacyclo octadecane and 4′-aminobenzo-18-crown-6, respectively, were prepared by the chemical immobilization of the ligand onto mesoporous silica support. The sorbents were characterized by FT-IR, scanning electron microscopy-energy dispersive X-ray microanalysis, elemental analysis and nitrogen adsorption-desorption test. The applicability of the sorbents for the extraction of biogenic amines by the batch sorption method was extensively studied and evaluated as a function of pH, biogenic amines concentration, contact time and reusability. Under the optimized conditions, all the sorbents exhibited highest selectivity toward spermidine (SPD) compared to other biogenic amines (tryptamine, putrescine, histamine and tyramine). Among the sorbents, AB18C6-MS offer the highest capacity and best selectivity towards SPD in the presence of other biogenic amines. The AB18C6-MS sorbent can be repeatedly used three times as there was no significant degradation in the extraction of the biogenic amines (%E > 85). The optimized procedure was successfully applied for the separation of SPD in food samples prior to the reversed-phase high performance liquid chromatography separation.     

Application of Ionic Liquid Modified Silica for Solid-Phase Extraction of Polysaccharides from Laminaria japonica

Silica-confined ionic liquids were synthesized for solid-phase extraction of polysaccharides, which was determined by high-performance liquid chromatography coupled with RI detection. The sorbent with amino-imidazolium groups was found to be the optimal material by a comparison of the adsorption capacity of fucoidan and laminarin onto different synthetic sorbents. The proper elution solvents for both laminarin and fucoidan were decided from practical tests. The sorbent performed stably and selectively, demonstrating potential applications in the separation of hydrophilic biomacromolecules, such as polysaccharides.     

Comparison of Hydrophilic Polymeric Sorbents for On-Line Solid-Phase Extraction of Polar Compounds from Aqueous Samples

Two 4-vinylimidazole-divinylbenzene (4VIm-DVB) polymers were synthesized and applied as sorbents for on-line solid-phase extraction (SPE) followed by liquid chromatography for analyzing polar compounds in aqueous samples. The new sorbents (4VIm-DVB) were compared to another sorbent that had been previously synthesized by our group (N-vinylimidazole-divinylbenzene (NVIm-DVB)) and to the commercial OASIS^® HLB and Strata^TM X. All the sorbents enabled 100 mL of sample to be on-line concentrated with good recoveries for the studied polar compounds. Real water samples were analyzed using NVIm-DVB and OASIS^® HLB as SPE sorbent, for which the best results were obtained.     

Affinity extraction of emerging contaminants from water based on bovine serum albumin as a binding agent

Affinity sorbents using bovine serum albumin as a binding agent were developed and tested for the extraction of environmental contaminants from water. Computer simulations based on a countercurrent distribution model were also used to study the behavior of these sorbents. Several model drugs, pesticides, and hormones of interest as emerging contaminants were considered in this work, with carbamazepine being used as a representative analyte when coupling the albumin column on‐line with liquid chromatography and tandem mass spectrometry. The albumin column was found to be capable of extracting carbamazepine from aqueous solutions that contained trace levels of this analyte. Further studies of the bovine serum albumin sorbent indicated that it had higher retention under aqueous conditions than a traditional C₁₈ support for most of the tested emerging contaminants. Potential advantages of using these protein‐based sorbents included the low cost of bovine serum albumin and its ability to bind to a relatively wide range of drugs and related compounds. It was also shown how simulations could be used to describe the elution behavior of the model compounds on the bovine serum albumin sorbents as an aid in optimizing the retention and selectivity of these supports for use with liquid chromatography or methods such as liquid chromatography with tandem mass spectrometry.     

Chitosan-silica nanocomposite sorbent for thin-layer chromatography of alkaloids

The feasibility of using a chitosan-silica nanocomposite sorbent in thin-layer chromatography of cytisine alkaloid and some of its derivatives was studied. The derivatives were obtained by the reactions of cytisine with aromatic aldehydes containing the -OH, -OCH₃, and -Br functional groups as substituents in different benzene ring positions. The separation of cytisine and its derivatives on the chitosan-silica sorbent was more effective than on initial silica gel. The mechanism of chromatographing on the two sorbents was considered; the mobile phase was a 6:1 (v/v) chloroform:methanol mixture.