Membrane-based techniques for sample enrichment

Sample preparation techniques based on non-porous membrane extraction generally offer a high degree of selectivity and enrichment power, together with convenient possibilities for direct and automated connections to chromatographic and other analytical instruments. In this review principles and applications for techniques as supported liquid membrane extraction, microporous membrane liquid-liquid extraction, polymeric membrane extraction and membrane extraction with a sorbent interface are described and compared.     

Capillary electrophoresis-based separation techniques for the analysis of proteins

CE offers the advantages of high speed, great efficiency, as well as the requirement of minimum amounts of sample and buffer for the analysis of proteins. In this review, we summarize the CE-based techniques coupled with absorption, LIF, and MS detection systems for the analysis of proteins mostly within the past 5 years. The basic principle of each technique and its advantages and disadvantages for protein analysis are discussed in brief. Advanced CE techniques, including on-column concentration techniques and high-efficiency multidimensional separation techniques, for high-throughput protein profiling of complex biological samples and/or of single cells are emphasized. Although the developed techniques provide improved peak capacity, they have not become practical tools for proteomics, mainly because of poor reproducibility, low-sample lading capacity, and low throughput due to ineffective interfaces between two separation dimensions and that between separation and MS systems. In order to identify the complexities and dynamics of the proteomes expressed by cells, tissues, or organisms, techniques providing improved analytical sensitivity, throughput, and dynamic ranges are still demanded.     

Membrane-based microextraction techniques in analytical chemistry: A review

The use of membrane-based sample preparation techniques in analytical chemistry has gained growing attention from the scientific community since the development of miniaturized sample preparation procedures in the 1990s. The use of membranes makes the microextraction procedures more stable, allowing the determination of analytes in complex and “dirty” samples. This review describes some characteristics of classical membrane-based microextraction techniques (membrane-protected solid-phase microextraction, hollow-fiber liquid-phase microextraction and hollow-fiber renewal liquid membrane) as well as some alternative configurations (thin film and electromembrane extraction) used successfully for the determination of different analytes in a large variety of matrices, some critical points regarding each technique are highlighted.     

Laboratory-based separation techniques for insoluble compound mixtures: methods for the purification of metal-organic framework materials

In this article, techniques for separating mixtures of insoluble compounds are discussed with respect to the small quantities found in laboratory preparations, as opposed to industrial quantities. The techniques include separations based on density, surface area and differences in particle size. Also discussed are simple apparatus, readily available in the laboratory or from commercial suppliers, for achieving these techniques.     

High-performance liquid chromatographic determination of morphine in biological samples: an overview of separation methods and detection techniques

High-performance liquid chromatogrpahy with electrochemical detection at present suits most of the needs of toxicologists for the determination of morphine and some related compounds in biological samples, although fluorescence detection is still a useful alternative. Chemiluminescence detection may be promising, but needs further optimization of its coupling with HPLC to give the best performances. Morphine detection by absorbance spectrophotometry does not seem to allow the degree of sensitivity and selectivity from matrix interferences that is required in most instances. However, this approach is useful when morphine congeners undetectable by alternative means (i.e., heroin and morphine-3-glucuronide) are to be determined or when a general toxicological screening is required.     

Development and analytical applications of multispectral imaging techniques: an overview

A multispectral imaging spectrometer is an instrument that can simultaneously record spectral and spatial information of a sample. Chemical and physical properties of the sample can be elucidated from such images. By synergistic use of an acousto-optic tunable filter and a progressive scan camera capable of snap shot recording it was possible to develop a novel imaging spectrometer with a spatial resolution of a few microns and which can record, grab and store up to 33 images per second (at a function of time) or 16 images per second (as a function of wavelength). This overview article summarizes the instrumentation development of various imaging spectrometers and their applications including its use as the detector for the determination of identity and sequences of peptides synthesized by the combinatorial solid phase method.     

Chiral separation in the class of proton pump inhibitors by chromatographic and electromigration techniques: An overview

Proton pump inhibitors (PPIs) are benzimidazole-derivative chiral sulfoxides, frequently used in the treatment of gastric hyperacidity-related disorders. Due to their stereoselective metabolism, the eutomeric forms of PPIs can present a more advantageous pharmacokinetic profile by comparison with the distomers or racemates. Moreover, two representatives of the class are used in therapy both as racemates and as pure enantiomers (esomeprazole, dexlansoprazole). A relatively large number of enantioseparation methods employed for the stereoselective determination of PPIs from pharmaceutical, biological, and environmental matrices were published in the past three decades. The purpose of the current overview is to provide a systematic survey of the available chiral separation methods published since the introduction of PPIs in the therapy up to the present. Analytical and bioanalytical methods using different chromatographic and electromigration techniques reported for the enantioseparation of omeprazole, lansoprazole, pantoprazole, rabeprazole, ilaprazole, and tenatoprazole are included. The analytical conditions of the presented methods are summarized in three comprehensive tables, while a critical discussion of the applied techniques, possible mechanism of enantiorecognition, and future perspectives on the topic are also presented.     

An overview on the application of ultrasound in extraction,separation and purification of plant polysaccharides

In view of the recent emphasis on non-conventional chemistry, application of ultrasound in isolation of plant polysaccharides represents a viable alternative to traditional extraction processes. This review presents an extensive literature survey of ultrasound-assisted extraction of polysaccharides from different plant materials, particularly herbal plants and secondary agricultural plant sources. Targeted, multistep methods were applied with respect to differences in the types of polysaccharides and their location in plant cell walls. The effectiveness of the methods was evaluated according to yield and properties of the isolated polysaccharides in comparison to classical extraction methods. Substantial shortening of extraction time, reduction of reagent consumption and/or extraction temperature are the most important advantages of the ultrasonic treatment. In combination with sequential extraction steps using different solvents, sonication was shown to be effective in separation and/or purification of polysaccharides. The disadvantages of the sonication treatment, such as degradation and compositional changes of the polysaccharide preparations are discussed as well.     

Imaging proteins with atomic force microscopy: an overview

Atomic force microscopy (AFM) has become a common tool for biophysical studies of proteins; mainly due its property to perform characterizations near physiological conditions. The tertiary and quaternary structures, forces driving folding-unfolding processes, and secondary structure elements can be studied in their native environments allowing high resolution level associated with small distortions. This review outlines the operational principles and applications of AFM for protein biophysics.     

Laser mass spectrometry: an overview of techniques,instruments and applications

Lasers have been used to produce intact molecular ions and structurally informative fragment ions of otherwise intractable biomolecules for examination by mass spectrometry. While laser microprobes have been used for this purpose, this paper focusses on other instrumental configurations, which require less focussed laser beams and which record ions that are produced by mechanisms which can be described thermodynamically. The time-of-flight and Fourier-transform ion-cyclotron resonance mass spectrometers emerge as the most suitable for use with pulsed laser desorption. Classes of compounds which are amenable to the technique include industrial polymers and carbohydrates.     

Commercialized rapid immunoanalytical tests for determination of allergenic food proteins: an overview

Food allergies have become an important health issue especially in industrialized countries. Undeclared allergenic ingredients or the presence of “hidden” allergens because of contamination during the food production process pose great health risks to sensitised individuals. The EU directive for food labelling lists allergenic foods that have to be declared on food products by the manufacturers. The list includes gluten-containing cereals, crustaceans, eggs, fish, peanuts, soybeans, milk, various nuts (e.g. almond, hazelnut, and walnut, etc.), celery, mustard, sesame seeds, lupin, and molluscs. Reliable methods for detection and quantification of food allergens are needed that can be applied in a fast and easy-to-use manner, are portable, and need only limited technical equipment. This review focuses on the latest developments in food allergen analysis with special emphasis on fast immunoanalytical methods such as rapid enzyme-linked immunosorbent assays (ELISA), lateral-flow immunochromatographic assays (LFA) and dipstick tests. Emerging technologies such as immunochemical microarrays and biosensors are also discussed and their application to food allergen analysis is reviewed. Finally, a comprehensive overview of rapid immunochemical test kits that are currently available commercially is given in tabular form.     

The effect of an organic eluent modifier and pH on the separation of wheat-storage proteins: Application to the purification of γ-gliadins ofTriticum monococcum L

Summary Reversed-phase, high-pressure liquid chromatography has been used to separate similar protein (γ-gliadin) components from 70% ethanol extracts of endosperm flour from two different accessions of the diploid wheatTriticum monococcum L. The effect of acetonitrile as the organic eluent was compared to acetonitrile: 2-propanol (3:1) at two different pH's. Conditions for maximum resolution of the γ-gliadin components were found to be at pH 7.2 with acetonitrile: 2-propanol (3:1) as the eluent. These conditions allowed the components to be obtained in sufficient purity for further charaterization. The mention of firm names or trade products does not imply that they are endorsed or recommended by the US Department of Agriculture over other firms or similar products not mentioned.     

Synthesis of an adsorbed reversed-phase packing material for the separation of proteins and peptides

We have described the preparation and chromatographic evaluation of an adsorbed hydrophobic stationary phase suitable for reversed-phase chromatography of proteins and peptides. The synthetic procedure involves three steps: the adsorption of a polyamine to the silica surface; crosslinking of the adsorbed polyamine layer with a bis-phenyl difunctional epoxide; and the benzoylation of the remaining accessible amino groups. Performance of this chromatographic material compared favorably with SynChropak RP-8 silica (SynChrom, Linden, IN, U.S.A.) and was stable to 40% formic acid. Good separations were obtained between the components of sample mixtures containing proteins or the cyanogen bromide fragments of sperm whale myoglobin. However, in both cases, the adsorbed hydrophobic stationary phase was less retentive. Furthermore, this medium exhibited slightly different selectivity. Whereas the heme which was present in the cyanogen bromide digest of myoglobin desorbed as the second peak from the RP-8 column, it eluted last from the adsorbed stationary phase. Comparable performance, acid stability and alternate selectivity suggest that this material is an interesting alternative to organosilane reversed-phase coatings.     

New agar microspheres for the separation and purification of natural products

A new type of agar chromatography media has been prepared with a yield over 80% using a water‐in‐oil emulsion technique. These microspheres have regular spherical shapes and particle diameters in the range 40–165 μm (average ～90 μm). Cross‐linking of the resulting agar microspheres with epichlorohydrin and 1,4‐butanediol diglycidyl ether enhanced their mechanical and thermal stability. The alkaline conditions used during the cross‐linking reaction also decreased the content of ionized sulfate groups of the polysaccharide, thus reducing the nonspecific adsorption of positively charged molecules. The cross‐linked agar microspheres were functionalized with (i) branched poly(ethyleneimine) to obtain a stationary phase useful for the separation of proteins in an anion‐exchange mode and (ii) with poly‐β‐cyclodextrin enabling direct isolation and purification of puerarin from a crude extract of Radix puerariae. Using a 23.5 mL column loaded with 20 mg extract (0.85 mg/mL gel), puerarin with a purity of 96% was recovered with a yield of 86%.     

外泌体分离与纯化技术研究进展

外泌体是所有真核细胞分泌到细胞外的直径介于30～150 nm的一种膜性纳米囊泡,参与细胞间生物信号的传递。大量实验证据表明,外泌体参与多种生物功能并发挥重要作用,包括蛋白质、RNA和脂质等生物分子的转移及多种疾病生理和病理过程的调节,被认为是疾病诊断、治疗和预后的重要的生物标志物和药物载体,因此发展简单、高效、经济的外泌体分离与纯化技术将有助于疾病的早期诊断和精准治疗。目前,利用外泌体的物理化学和生物化学特性已开发出多种分离外泌体的技术,但仍缺乏标准化和规模化临床级外泌体的分离方法,从而限制了其临床应用。另外,对分离出的外泌体的特征、纯度和数量的鉴定是判断外泌体分离纯化方法优劣的重要指标。本文综述了外泌体分离与纯化技术以及鉴定方法的研究进展,主要讨论分离技术的机制、性能、挑战和前景以及外泌体的鉴定方法,以期为外泌体的分离纯化提供新的思路和解决策略。     

Kinetic approach for the purification of nucleotides with magnetic separation

The isolation of β‐nicotinamide adenine dinucleotide is of great importance since it is widely used in different scientific and technologic fields such as biofuel cells, sensor technology, and hydrogen production. In order to isolate β‐nicotinamide adenine dinucleotide, first 3‐aminophenyboronic acid functionalized magnetic nanoparticles were prepared to serve as a magnetic solid support and subsequently they were used for reversible adsorption/desorption of β‐nicotinamide adenine dinucleotide in a batch fashion. The loading capacity of the 3‐aminophenyboronic acid functionalized nanoparticles for β‐nicotinamide adenine dinucleotide adsorption was 13.0 μmol/g. Adsorption kinetic and isotherm studies showed that the adsorption process followed a pseudo‐second‐order kinetic model and the experimental data can be represented using Langmuir isotherm model. The 3‐aminophenyboronic acid functionalized magnetic nanoparticles were proposed as an alternative support for the β‐nicotinamide adenine dinucleotide purification. The results elucidated the significance of magnetic separation as a fast, relatively simple, and low‐cost technique. Furthermore, the magnetic supports can be reused at least five times for purification processes.