Free-flow electrophoresis

Last updated August 01, 2024

Free-flow electrophoresis (FFE), also known as carrier-free electrophoresis, is a matrix-free, high-voltage electrophoretic separation technique. FFE is an analogous technique to capillary electrophoresis, with a comparable resolution, that can be used for scientific questions, where semi-preparative and preparative amounts of samples are needed. It is used to quantitatively separate samples according to differences in charge or isoelectric point by forming a pH gradient. Because of the versatility of the technique, a wide range of protocols for the separation of samples like rare metal ions, protein isoforms, multiprotein complexes, peptides, organelles, cells, DNA origami, blood serum and nanoparticles exist. The advantage of FFE is the fast and gentle separation of samples dissolved in a liquid solvent without any need of a matrix, like polyacrylamide in gel electrophoresis. This ensures a very high recovery rate since analytes do not adhere to any carrier or matrix structure. Because of its continuous nature and high volume throughput, this technique allows a fast separation of preparative amounts of samples with a very high resolution. Furthermore, the separations can be conducted under native or denaturing conditions.^[1]

History

FFE was developed in the 1960s by Kurt Hannig at the Max-Planck-Institute in Germany.^[2] Until the 1980s, it was a standardized technology for the separation of cells and organelles, and FFE was even tested in space to minimize the sedimentation under zero gravity.^[3] As flow cytometry became the standard method for cell sorting, FFE developments focused on the separation of proteins and charged particles. Some groups are also working on miniaturized versions of FFE systems or micro FFEs.^[4]

Technique

The separation chamber consists of a backplate and a front plate. The backplate usually consists of a cooled aluminum block, covered with a plastic covered glass mirror. The front plate is nowadays made of PMMA, in earlier times glass has been used. The distance between the front- and the backplate can be adjusted by spacers and is usually between 0.1–0.5 mm. The front plate also contains the inlets for the separation buffers and the sample, the outlets for the fractionation tubes and the platinum wires as electrodes. By applying different buffers over the multiple buffer inlets the operator is able to change pH, salt concentrations or composition and therefore the separation conditions over the width of the chamber. The separation buffers and the sample are applied by peristaltic pumps, to ensure a laminar flow. A high voltage electric field is applied perpendicular to the laminar flow. Analytes in the laminar flow can be separated by charge density and isoelectric point. Because of its highly versatile nature, this technique can make use of different modes of electrophoresis, like for example isotachophoresis, isoelectric focusing or (interval) zone electrophoresis. ^{[ citation needed ]}

At the end of the separation cell, the separated sample is split up at the fractionation tubes and collected in microtiter plates.^[5]

Schematic functionality of Free Flow Electrophoresis

Afterwards the samples can be characterized by all major techniques like HPLC, LC-MS, mass spectrometry (ESI / MALDI, depending on the protocol used) or electrophoresis (IEF / SDS PAGE, 2D-PAGE).^{[ citation needed ]}

Applications

Standard application include the high-resolution separation of protein complexes, membrane proteins, protein and antibody isoforms, cells, subcellular compartments (like organelles, ribosomes) and liposomes.^[6] By making use of very flat pH-gradients, generated by ampholytes, it is possible to separate protein isoforms, that vary by less than 0.02 pH units, with a throughput of around 3 mg/h.^[7] It is also possible to add additives to the buffers to increase the resolution or denature the samples. Typically concentrations of urea up to 8M, 0.1–1% of detergents like: CHAPS, CHAPSO, Digitonin, Dodecyl-ß-D-maltoside, Octyl-ß-D-glucoside, Triton-X-114 (IEF) and DTT up to 50 mM are tolerated.^{[ citation needed ]}

Key features

Matrix free separation, ideal for conserving protein activity/protein complexes
High resolution separation of protein complexes, membrane proteins, protein isoforms, cells, subcellular compartments (like organelles, ribosomes, etc.),
Separation size range from ions to complete cells
Sample recovery up to 99%, depending on sample and mode of operation
High reproducibility of individual runs
Separation in several minutes
Protocols for Isoelectric Focusing separation with different commercial ampholytes and atoxic small molecular ProLytesTM for direct clinical application
Fast and sensitive detection of separation quality via UV, IEF-gels
Compatible with many other downstream techniques, e.g. HPLC, MS, SDS-, IEF- and 2D-GE
Suited for separation of unstable proteins due to cooling of samples and separation chamber down to 4 °C
Reduction of the complexity of the proteome before further proteomic analysis^[8]
Enriching low-abundant proteins by removing excess of unwanted proteins
Compatible with large and small sample volumes from around 50 μL up to several milliliters.
Preparative as well as analytical operation modes
Supports all electrophoretic separation modes (IEF, IZE, ZE, ITP)
Can be run under native or denaturing conditions

Related Research Articles

<span class="mw-page-title-main">Agarose gel electrophoresis</span> Method for separation and analysis of biomolecules using agarose gel

Agarose gel electrophoresis is a method of gel electrophoresis used in biochemistry, molecular biology, genetics, and clinical chemistry to separate a mixed population of macromolecules such as DNA or proteins in a matrix of agarose, one of the two main components of agar. The proteins may be separated by charge and/or size, and the DNA and RNA fragments by length. Biomolecules are separated by applying an electric field to move the charged molecules through an agarose matrix, and the biomolecules are separated by size in the agarose gel matrix.

Gel electrophoresis is a method for separation and analysis of biomacromolecules and their fragments, based on their size and charge. It is used in clinical chemistry to separate proteins by charge or size and in biochemistry and molecular biology to separate a mixed population of DNA and RNA fragments by length, to estimate the size of DNA and RNA fragments or to separate proteins by charge.

The isoelectric point (pI, pH(I), IEP), is the pH at which a molecule carries no net electrical charge or is electrically neutral in the statistical mean. The standard nomenclature to represent the isoelectric point is pH(I). However, pI is also used. For brevity, this article uses pI. The net charge on the molecule is affected by pH of its surrounding environment and can become more positively or negatively charged due to the gain or loss, respectively, of protons (H⁺).

<span class="mw-page-title-main">Polyacrylamide gel electrophoresis</span> Analytical technique

Polyacrylamide gel electrophoresis (PAGE) is a technique widely used in biochemistry, forensic chemistry, genetics, molecular biology and biotechnology to separate biological macromolecules, usually proteins or nucleic acids, according to their electrophoretic mobility. Electrophoretic mobility is a function of the length, conformation, and charge of the molecule. Polyacrylamide gel electrophoresis is a powerful tool used to analyze RNA samples. When polyacrylamide gel is denatured after electrophoresis, it provides information on the sample composition of the RNA species.

The western blot, or western blotting, is a widely used analytical technique in molecular biology and immunogenetics to detect specific proteins in a sample of tissue homogenate or extract. Besides detecting the proteins, this technique is also utilized to visualize, distinguish, and quantify the different proteins in a complicated protein combination.

<span class="mw-page-title-main">Two-dimensional gel electrophoresis</span> Form of gel electrophoresis used in analyzing proteins

Two-dimensional gel electrophoresis, abbreviated as 2-DE or 2-D electrophoresis, is a form of gel electrophoresis commonly used to analyze proteins. Mixtures of proteins are separated by two properties in two dimensions on 2D gels. 2-DE was first independently introduced by O'Farrell and Klose in 1975.

Protein purification is a series of processes intended to isolate one or a few proteins from a complex mixture, usually cells, tissues or whole organisms. Protein purification is vital for the specification of the function, structure and interactions of the protein of interest. The purification process may separate the protein and non-protein parts of the mixture, and finally separate the desired protein from all other proteins. Ideally, to study a protein of interest, it must be separated from other components of the cell so that contaminants will not interfere in the examination of the protein of interest's structure and function. Separation of one protein from all others is typically the most laborious aspect of protein purification. Separation steps usually exploit differences in protein size, physico-chemical properties, binding affinity and biological activity. The pure result may be termed protein isolate.

<span class="mw-page-title-main">Gel electrophoresis of proteins</span> Technique for separating proteins

Protein electrophoresis is a method for analysing the proteins in a fluid or an extract. The electrophoresis may be performed with a small volume of sample in a number of alternative ways with or without a supporting medium, namely agarose or polyacrylamide. Variants of gel electrophoresis include SDS-PAGE, free-flow electrophoresis, electrofocusing, isotachophoresis, affinity electrophoresis, immunoelectrophoresis, counterelectrophoresis, and capillary electrophoresis. Each variant has many subtypes with individual advantages and limitations. Gel electrophoresis is often performed in combination with electroblotting or immunoblotting to give additional information about a specific protein.

Isoelectric focusing (IEF), also known as electrofocusing, is a technique for separating different molecules by differences in their isoelectric point (pI). It is a type of zone electrophoresis usually performed on proteins in a gel that takes advantage of the fact that overall charge on the molecule of interest is a function of the pH of its surroundings.

Micellar electrokinetic chromatography (MEKC) is a chromatography technique used in analytical chemistry. It is a modification of capillary electrophoresis (CE), extending its functionality to neutral analytes, where the samples are separated by differential partitioning between micelles and a surrounding aqueous buffer solution.

Capillary electrophoresis (CE) is a family of electrokinetic separation methods performed in submillimeter diameter capillaries and in micro- and nanofluidic channels. Very often, CE refers to capillary zone electrophoresis (CZE), but other electrophoretic techniques including capillary gel electrophoresis (CGE), capillary isoelectric focusing (CIEF), capillary isotachophoresis and micellar electrokinetic chromatography (MEKC) belong also to this class of methods. In CE methods, analytes migrate through electrolyte solutions under the influence of an electric field. Analytes can be separated according to ionic mobility and/or partitioning into an alternate phase via non-covalent interactions. Additionally, analytes may be concentrated or "focused" by means of gradients in conductivity and pH.

<span class="mw-page-title-main">Molecular-weight size marker</span> Set of standards

A molecular-weight size marker, also referred to as a protein ladder, DNA ladder, or RNA ladder, is a set of standards that are used to identify the approximate size of a molecule run on a gel during electrophoresis, using the principle that molecular weight is inversely proportional to migration rate through a gel matrix. Therefore, when used in gel electrophoresis, markers effectively provide a logarithmic scale by which to estimate the size of the other fragments.

QPNC-PAGE, or QuantitativePreparativeNativeContinuousPolyacrylamideGel Electrophoresis, is a bioanalytical, one-dimensional, high-resolution and high-precision electrophoresis technique applied in biochemistry and bioinorganic chemistry to separate proteins quantitatively by isoelectric point and by continuous elution from a gel column.

Within chemistry for acid–base reactions, Immobilized pH gradient (IPG) gels are the acrylamide gel matrix co-polymerized with the pH gradient, which result in completely stable gradients except the most alkaline (>12) pH values. The immobilized pH gradient is obtained by the continuous change in the ratio of Immobilines. An Immobiline is a weak acid or base defined by its pK value. Immobilized pH gradients (IPG) are made by mixing two kinds of acrylamide mixture, one with Immobiline having acidic buffering property and other with basic buffering property. The concentrations of the buffers in the two solutions define the range and shape of the pH gradient produced. Both solutions contain acrylamide monomers and catalysts. During polymerization, the acrylamide portion of the buffers co polymerize with the acrylamide and bisacrylamide monomers to form a polyacrylamide gel. These polymerised gels are backed with plastic based backing that allow ease in handling and improve IPG's performance. The gel is then washed to remove catalysts and unpolymerized monomers, which interfere with isoelectric separation. IPG increased reproducibility of isoelectric focusing and 2D-gel electrophoresis. Other advantages are increased resolution, reproducible separation of alkaline proteins and increased loading capacity.

<span class="mw-page-title-main">Bio-MEMS</span>

Bio-MEMS is an abbreviation for biomedical microelectromechanical systems. Bio-MEMS have considerable overlap, and is sometimes considered synonymous, with lab-on-a-chip (LOC) and micro total analysis systems (μTAS). Bio-MEMS is typically more focused on mechanical parts and microfabrication technologies made suitable for biological applications. On the other hand, lab-on-a-chip is concerned with miniaturization and integration of laboratory processes and experiments into single chips. In this definition, lab-on-a-chip devices do not strictly have biological applications, although most do or are amenable to be adapted for biological purposes. Similarly, micro total analysis systems may not have biological applications in mind, and are usually dedicated to chemical analysis. A broad definition for bio-MEMS can be used to refer to the science and technology of operating at the microscale for biological and biomedical applications, which may or may not include any electronic or mechanical functions. The interdisciplinary nature of bio-MEMS combines material sciences, clinical sciences, medicine, surgery, electrical engineering, mechanical engineering, optical engineering, chemical engineering, and biomedical engineering. Some of its major applications include genomics, proteomics, molecular diagnostics, point-of-care diagnostics, tissue engineering, single cell analysis and implantable microdevices.

Capillary electrophoresis–mass spectrometry (CE–MS) is an analytical chemistry technique formed by the combination of the liquid separation process of capillary electrophoresis with mass spectrometry. CE–MS combines advantages of both CE and MS to provide high separation efficiency and molecular mass information in a single analysis. It has high resolving power and sensitivity, requires minimal volume and can analyze at high speed. Ions are typically formed by electrospray ionization, but they can also be formed by matrix-assisted laser desorption/ionization or other ionization techniques. It has applications in basic research in proteomics and quantitative analysis of biomolecules as well as in clinical medicine. Since its introduction in 1987, new developments and applications have made CE-MS a powerful separation and identification technique. Use of CE–MS has increased for protein and peptides analysis and other biomolecules. However, the development of online CE–MS is not without challenges. Understanding of CE, the interface setup, ionization technique and mass detection system is important to tackle problems while coupling capillary electrophoresis to mass spectrometry.

<span class="mw-page-title-main">Affinity electrophoresis</span>

Affinity electrophoresis is a general name for many analytical methods used in biochemistry and biotechnology. Both qualitative and quantitative information may be obtained through affinity electrophoresis. Cross electrophoresis, the first affinity electrophoresis method, was created by Nakamura et al. Enzyme-substrate complexes have been detected using cross electrophoresis. The methods include the so-called electrophoretic mobility shift assay, charge shift electrophoresis and affinity capillary electrophoresis. The methods are based on changes in the electrophoretic pattern of molecules through biospecific interaction or complex formation. The interaction or binding of a molecule, charged or uncharged, will normally change the electrophoretic properties of a molecule. Membrane proteins may be identified by a shift in mobility induced by a charged detergent. Nucleic acids or nucleic acid fragments may be characterized by their affinity to other molecules. The methods have been used for estimation of binding constants, as for instance in lectin affinity electrophoresis or characterization of molecules with specific features like glycan content or ligand binding. For enzymes and other ligand-binding proteins, one-dimensional electrophoresis similar to counter electrophoresis or to "rocket immunoelectrophoresis", affinity electrophoresis may be used as an alternative quantification of the protein. Some of the methods are similar to affinity chromatography by use of immobilized ligands.

Discontinuous electrophoresis is a type of polyacrylamide gel electrophoresis. It was developed by Ornstein and Davis. This method produces high resolution and good band definition. It is widely used technique for separating proteins according to size and charge.

SDS-PAGE is a discontinuous electrophoretic system developed by Ulrich K. Laemmli which is commonly used as a method to separate proteins with molecular masses between 5 and 250 kDa. The combined use of sodium dodecyl sulfate and polyacrylamide gel eliminates the influence of structure and charge, and proteins are separated by differences in their size. At least up to 2012, the publication describing it was the most frequently cited paper by a single author, and the second most cited overall.

Pier Giorgio Righetti is a professor emeritus of chemistry. He worked primarily at the University of Milano (1971-1995) and at the Department of Chemistry of the Politecnico di Milano in Milan, Italy (2005-2011). He has served as the President of the Società Italiana di Proteomica.

References

↑ P.D. Patel and G. Weber, Electrophoresis in free fluid: a review of the technology and agrifood applications, J. Biol. Phys. Chem. 2003, 3, 60–73.
↑ Free Flow Elektrophoresis, Kurt Hannig und Hans G. Heidrich, GIT Verlag 1990, ISBN 3-921956-88-9
↑ Electrophoresis in Space – 1985, PDF
↑ S. Jezierski, L. Gitlin, S. Nagl, D. Belder, Multistep liquid-phase lithography for fast prototyping of microfluidic free-flow-electrophoresis chips, Anal. Bioanal. Chem., 2011, 401, 2651-2656.
↑ "Principle of FFE separations". Archived from the original on 2014-12-01. Retrieved 2013-06-04.
↑ "Applications of Free Flow Electrophoresis". Archived from the original on 2018-11-16. Retrieved 2019-01-21.
↑ "Archived copy" (PDF). Archived from the original (PDF) on 2016-03-04. Retrieved 2016-01-12.{{cite web}}: CS1 maint: archived copy as title (link)
↑ Islinger, M; Eckerskorn, C; Völkl, A (2010). "Free-flow electrophoresis in the proteomic era: a technique in flux". Electrophoresis. 31 (11): 1754–63. doi:10.1002/elps.200900771. PMID 20506416. S2CID 28034848.

External links

This page is based on this Wikipedia article
Text is available under the CC BY-SA 4.0 license; additional terms may apply.
Images, videos and audio are available under their respective licenses.

[Patel-1] P.D. Patel and G. Weber, Electrophoresis in free fluid: a review of the technology and agrifood applications, J. Biol. Phys. Chem. 2003, 3, 60–73.

[2] Free Flow Elektrophoresis, Kurt Hannig und Hans G. Heidrich, GIT Verlag 1990, ISBN 3-921956-88-9

[3] Electrophoresis in Space – 1985, PDF

[4] S. Jezierski, L. Gitlin, S. Nagl, D. Belder, Multistep liquid-phase lithography for fast prototyping of microfluidic free-flow-electrophoresis chips, Anal. Bioanal. Chem., 2011, 401, 2651-2656.

[5] "Principle of FFE separations". Archived from the original on 2014-12-01. Retrieved 2013-06-04.

[6] "Applications of Free Flow Electrophoresis". Archived from the original on 2018-11-16. Retrieved 2019-01-21.

[7] "Archived copy" (PDF). Archived from the original (PDF) on 2016-03-04. Retrieved 2016-01-12.{{cite web}}: CS1 maint: archived copy as title (link)

[8] Islinger, M; Eckerskorn, C; Völkl, A (2010). "Free-flow electrophoresis in the proteomic era: a technique in flux". Electrophoresis. 31 (11): 1754–63. doi:10.1002/elps.200900771. PMID 20506416. S2CID 28034848.

[1]

[2]

[3]

[4]

[5]

[6]

[7]

[8]