Dialysis-assisted two-dimensional gel electrophoresis

2-DE is an important tool in proteomics research. However, intrinsic gel-to-gel variability of 2-DE often masks the biological differences between the samples and compromises quantitative comparison of protein expression levels. Here, we describe a modification of 2-DE that results in improved matching and quantification of proteins. This was accomplished by performing IEF of two samples in two IPG strips separated by a dialysis membrane. After IEF running, the strips were separated and the SDS-PAGE dimension was accomplished on two individual gels. After gel staining with CBB, ImageMaster 2D Platinum software (Amersham) was used for spot detection and quantification. Analysis of protein extracts from C2C12 myoblasts by this method resulted in 99% spot-matching efficiency and CV in stain intensity (% volume) was less than 0.5 for 98% of spots. We conclude that this technique, called dialysis-assisted gel electrophoresis, gives superior spot matching and quantitative reproducibility compared to IEF conducted on separate strips.     

Functionalization of cellulose dialysis membranes for chiral separation using beta-cyclodextrin immobilization

A membrane-based chiral separation system for the separation of racemic tryptophan solutions is developed by the covalently binding beta-cyclodextrin onto the surface of commercial cellulose membranes. The immobilization process is monitored by XPS. AFM demonstrates the evolutionary transition of membrane surface morphology before and after the CD immobilization. Due to their different complexation with immobilized CD, dialysis transport experiments show d-tryptophan preferential permeability through the immobilized CD membranes, and the enantioselectivity is 1.10. A model based on the existence of a thin chiral solution layer of amino acid at the interface between the feed solution and the membrane has been proposed. This chiral separation model has been verified using the chiral separation results of racemic amino acids and binding constants of amino acids with CD. The effect of membrane's pore size on enantioselectivity has also been investigated. The immobilized CD membrane, having MWCO 1000, exhibits the highest enantioselectivity to the racemic tryptophan solution.     

Optimization of a flow injection analysis system for tartaric acid determination in wines

The objective of this work is the development and optimization of a method for tartaric acid analysis in wines that does not require any sample pre-treatment and with adequate accuracy. A flow injection analysis manifold with three channels, using a dialysis unit to eliminate sample matrix interferences and to accomplish on-line dilution, is proposed for the spectrophotometrical determination of tartaric acid in wines making use of its reaction with vanadate. The proposed method is fast, accurate, simple, economic and does not require any sample pre-treatment. Preliminary studies using factorial designs were performed to determine which operational parameters should be included in the optimization stage. The optimization was performed using a modified simplex algorithm with a response function that included sensitivity, deviation from linearity at low concentrations and residence time, used as an inverse measure of sampling rate. The most relevant analytical parameters of the method are presented, including a comparison between the results provided by the proposed method and by an alternative procedure in the analysis of a set of wine samples from Portugal, with tartaric acid values in the range 0.5–4 g l⁻¹.     

Separation/preconcentration of trace heavy metals in urine, sediment and dialysis concentrates by coprecipitation with samarium hydroxide for atomic absorption spectrometry

Multi-element determination of trace elements in urine and dialysis solutions by atomic absorption spectrometry has been investigated. Coprecipitation with samarium hydroxide was used for preconcentration of trace elements and elimination of matrix elements. To 10 ml of each sample was added 500 μl of 2 mg ml⁻¹ samarium solutions; the pH was then adjusted to 12.2 in order to collect trace heavy metals on samarium hydroxide. The precipitate was separated by centrifugation and dissolved in 1 ml of 1 mol l⁻¹ HNO₃. Coprecipitation parameters and matrix effects are discussed. The precision, based on replicate analysis, is around 5% for the analytes, and recovery is quantitative, based on analysis of spiked samples and solutions including matrix components. The time required for the coprecipitation and determination was about 30 min.     

Nanotechnological evaluation of protein adsorption on dialysis membrane surface hydrophilized with polyvinylpyrrolidone

Hydrophilizing synthetic polymer dialysis membranes with polyvinylpyrrolidone (PVP) play an important role for inhibition of protein adsorption on membrane surface. In the present study, the effect of PVP on protein adsorption was evaluated from a nano-scale perspective. Swelling behavior of PVP present on wet polysulfone (PS)/PVP film surfaces was observed by atomic force microscopy (AFM). Fibrinogen and human serum albumin (HSA) were immobilized on the tip of AFM probes, with which a force-curve between protein and wet PS/PVP film surface was measured by AFM while scanning in order to visualize two-dimensional protein adsorbability on film surfaces. Furthermore, HSA adsorbability on non-PVP containing PEPA dialysis membrane (FLX-15GW) and PVP containing PEPA dialysis membrane (FDX-150GW) was evaluated by the AFM force-curve method. As a result, PS/PVP film surface was completely covered with hydrated and swollen PVP at 5 wt% or more PVP content. Protein adsorbability on PS/PVP film surfaces decreased greatly with increasing content of PVP. The adsorption of HSA was inhibited by the presence of PVP on film surfaces more significantly than that of more hydrophobic fibrinogen. HSA adsorbability on wet FLX-15GW dialysis membrane surface was 428 ± 174 pN whereas that on wet FDX-150GW dialysis membrane surface was 42 ± 29 pN.     

Continuous Amperometric Determination of Glucose Using an Immobilized Enzyme Reactor in Combination with an Immersible Dialysis Probe

Abstract

Glucose was continuously determined by reaction in a packed-bed enzyme reactor containing glucose oxidase and catalase. Oxygen consumption was measured amperometrically with a polarographic Clark electrode. Glucose was sampled through a dialysis probe immersed in the solution to be measured. An extension of the normal range for the enzyme was achieved by modulating the flow rate through the dialysis probe and a linear response was obtained in the range of 1.0-60 mM glucose. The correlation between the glucose transfer and the membrane area of the dialysis probe was also studied. Six different membranes were used, all showing variations in the adhesion of yeast cells.     

Fully automated column-switching HPLC determination of aflatoxin M1 in milk using dialysis as sample preparation

A procedure has been developed for the automated determination of aflatoxin M1 in decreamed milk, by using on-line dialysis and subsequent trace enrichment on a reverse phase column. After foreflush to the analytical column the determination is performed with fluorescence detection. Fully automated analysis within 10 min is thus possible with reproducible dialysis recoveries above 50% (CV is 3.3%, n = 20) and detection levels of 50 ng/kg.     

Characterization of Zinc Ion Transport Via Dialysis Process

Treatment of metal ions' wastes is getting more interest due to the tight regulations for environmental protection. Dialysis, a membrane based process with the concentration difference as the driving force, may be used for separation of metal ions from wastewater. In this study membranes with different pore sizes including Accurel, Celgard, GVHP, PM30 and PTHK membranes were employed to characterise the transport of zinc ion in various (0.01, 0.1, 0.5, 1, 5 and 10 w/v percent) initial feed concentrations. The results show that low initial feed concentration causes less passage of ions through the membrane due to low driving force, i.e. concentration gradient across the membrane. This result is expected. However the effect of membrane pore size is somehow unexpected. It was found that the large pore size membranes provide less penetration of the metal ions through the membrane. This reproducible result has been explained based on the transport mechanism. Two types of mechanisms, i.e. extensive and intensive mechanisms, have been suggested for metal ion transport through different pore size membranes.     

Coupling on-line of a dialyser with a flow-continuous system to separate Vitamin B(12) from milk

The use of membranes for on-line separations in flow-through dialyser as a part of a flow system is extremely useful for automated samples preparation. In this paper a method to couple the dialysis and the UV detection on-line of Vitamin B₁₂ from milk is proposed. Firstly, the milk samples were pre-treated with trichloroacetic and centrifuged (to eliminate proteins and fats) and later, using a dialyser coupled a flow-continuous manifold was possible dialyse the Vitamin B₁₂, which was monitored spectrophotometrically at 361 nm. On the other hand, the milk samples were also dialysed on-line but without the acid treatment and the results were compared. The influence of various parameters, including the pump speed for both the donor and acceptor stream, dialysis time, donor and acceptor loop volume on dialysis efficiency was studied. The method was applied to different kinds of milk (skimmed and semi-skimmed milk, evaporated milk, lactose free milk and liquid and powder whole milk). The relative standard deviation (R.S.D.) of the proposed method was of 0.45% and the obtained dialysis percentage was of 5.8%. The proposed method very easy permit a pre-treatment of the sample, quick and on-line with the detection. The dialysis process permitted the pass of vitamin and avoided the pass of other analytes as proteins in the case of the milk samples without acid treatment.     

A high-efficiency sample introduction system for capillary electrophoresis analysis of amino acids from dynamic samples and static dialyzed human vitreous samples

A low-volume automated injection system for the analysis of chemically complex, amino acid samples is presented. This system utilizes submicroliter sample volumes stored on a 75-μm inner diameter capillary. A pulse of positive pressure (82 kPa) is used to load nanoliter sample volumes into an in-house fabricated interface and onto a separation capillary. Residual sample solution in the interface is immediately washed away by a continuous transverse flow through the injection interface, yielding a sharp and reproducible sample plug. By performing multiple injections of a static sample, one may average the signals to yield a signal-to-noise ratio improvement of up to 4.07-fold for 20 injections compared with a theoretical maximum of a 4.47-fold improvement. Without interruption of the applied voltage, injections performed every 150 s were used to monitor the progress of the reaction of multiple amino acids with the fluorogenic dye 3-(4-carboxybenzoyl)quinoline-2-carboxaldehyde. Analysis of dialyzed clinical vitreous samples demonstrates the resolution and quantitation of arginine, lysine, leucine, glutamine, and glutamate. Observed levels are comparable with those of nonautomated injection methods and reports by others. Figure Multiple injections of fluorescently labeled human vitreous with a detailed view of a single injection (above) and with all injections segmented and averaged for signal-to-noise ratio improvement (right)