Gel
electrophoresis apparatus – an agarose gel is placed in this
buffer-filled box and an electrical field is applied via the power
supply to the rear. The negative terminal is at the far end (black
wire), so DNA migrates toward the positively charged anode (red wire).
| |
| Classification | Electrophoresis |
|---|---|
| Other techniques | |
| Related | Capillary electrophoresis SDS-PAGE Two-dimensional gel electrophoresis Temperature gradient gel electrophoresis |
Digital
image of 3 plasmid restriction digests run on a 1% w/v agarose gel, 3
volt/cm, stained with ethidium bromide. The DNA size marker is a
commercial 1 kbp ladder. The position of the wells and direction of DNA
migration is noted.
The
image above shows how small DNA fragments will migrate through agarose
gel farther than large DNA fragments during electrophoresis. The graph
to the right shows the nonlinear, relationship between the size of the
DNA fragment and the distance migrated.
Gel
Electrophoresis is a process where an electric current is applied to
DNA samples creating fragments that can be used for comparison between
DNA samples.
1) DNA is extracted.
2) Isolation and amplification of DNA.
3) DNA added to the gel wells.
4) Electric current applied to the gel.
5) DNA bands are separated by size.
6) DNA bands are stained.
1) DNA is extracted.
2) Isolation and amplification of DNA.
3) DNA added to the gel wells.
4) Electric current applied to the gel.
5) DNA bands are separated by size.
6) DNA bands are stained.
Gel electrophoresis is a method for separation and analysis of macromolecules (DNA, RNA and proteins)
and their fragments, based on their size and charge. It is used in
clinical chemistry to separate proteins by charge or size (IEF agarose,
essentially size independent) 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.
Nucleic acid molecules are separated by applying an electric field to move the negatively charged molecules through a matrix of agarose
or other substances. Shorter molecules move faster and migrate farther
than longer ones because shorter molecules migrate more easily through
the pores of the gel. This phenomenon is called sieving.
Proteins are separated by charge in agarose because the pores of the
gel are too large to sieve proteins. Gel electrophoresis can also be
used for separation of nanoparticles.
Gel electrophoresis uses a gel as an anticonvective medium or
sieving medium during electrophoresis, the movement of a charged
particle in an electrical field. Gels suppress the thermal convection
caused by application of the electric field, and can also act as a
sieving medium, retarding the passage of molecules; gels can also simply
serve to maintain the finished separation, so that a post
electrophoresis stain can be applied. DNA Gel electrophoresis is usually performed for analytical purposes, often after amplification of DNA via polymerase chain reaction (PCR), but may be used as a preparative technique prior to use of other methods such as mass spectrometry, RFLP, PCR, cloning, DNA sequencing, or Southern blotting for further characterization.
Physical basis
Overview of Gel Electrophoresis.
Electrophoresis
is a process which enables the sorting of molecules based on size.
Using an electric field, molecules (such as DNA) can be made to move
through a gel made of agarose or polyacrylamide.
The electric field consists of a negative charge at one end which
pushes the molecules through the gel, and a positive charge at the other
end that pulls the molecules through the gel. The molecules being
sorted are dispensed into a well in the gel material. The gel is placed
in an electrophoresis chamber, which is then connected to a power
source. When the electric current is applied, the larger molecules move
more slowly through the gel while the smaller molecules move faster. The
different sized molecules form distinct bands on the gel.
The term "gel" in this instance refers to the matrix used to contain, then separate the target molecules. In most cases, the gel is a crosslinked polymer
whose composition and porosity is chosen based on the specific weight
and composition of the target to be analyzed. When separating proteins or small nucleic acids (DNA, RNA, or oligonucleotides) the gel is usually composed of different concentrations of acrylamide and a cross-linker, producing different sized mesh networks of polyacrylamide. When separating larger nucleic acids (greater than a few hundred bases),
the preferred matrix is purified agarose. In both cases, the gel forms a
solid, yet porous matrix. Acrylamide, in contrast to polyacrylamide, is
a neurotoxin
and must be handled using appropriate safety precautions to avoid
poisoning. Agarose is composed of long unbranched chains of uncharged
carbohydrate without cross links resulting in a gel with large pores
allowing for the separation of macromolecules and macromolecular complexes.
Electrophoresis refers to the electromotive force
(EMF) that is used to move the molecules through the gel matrix. By
placing the molecules in wells in the gel and applying an electric
field, the molecules will move through the matrix at different rates,
determined largely by their mass when the charge-to-mass ratio (Z) of
all species is uniform. However, when charges are not all uniform the
electrical field generated by the electrophoresis procedure will cause
the molecules to migrate differentially according to charge. Species
that are net positively charged will migrate towards the cathode which is negatively charged (because this is an electrolytic rather than galvanic cell),
whereas species that are net negatively charged will migrate towards
the positively charged anode. Mass remains a factor in the speed with
which these non-uniformly charged molecules migrate through the matrix
toward their respective electrodes.
If several samples have been loaded into adjacent wells in the
gel, they will run parallel in individual lanes. Depending on the number
of different molecules, each lane shows separation of the components
from the original mixture as one or more distinct bands, one band per
component. Incomplete separation of the components can lead to
overlapping bands, or to indistinguishable smears representing multiple
unresolved components.
Bands in different lanes that end up at the same distance from the top
contain molecules that passed through the gel with the same speed,
which usually means they are approximately the same size. There are molecular weight size markers
available that contain a mixture of molecules of known sizes. If such a
marker was run on one lane in the gel parallel to the unknown samples,
the bands observed can be compared to those of the unknown in order to
determine their size. The distance a band travels is approximately
inversely proportional to the logarithm of the size of the molecule.
There are limits to electrophoretic techniques. Since passing
current through a gel causes heating, gels may melt during
electrophoresis. Electrophoresis is performed in buffer solutions to
reduce pH changes due to the electric field, which is important because
the charge of DNA and RNA depends on pH, but running for too long can
exhaust the buffering capacity of the solution. There are also
limitations in determining the molecular weight by SDS-PAGE, especially
when trying to find the MW of an unknown protein. There are certain
biological variables that are difficult or impossible to minimize and
can affect the electrophoretic migration. Such factors include protein
structure, post-translational modifications, and amino acid composition.
For example, tropomyosin is an acidic protein that migrates abnormally
on SDS-PAGE gels. This is because the acidic residues are repelled by
the negatively charged SDS, leading to an inaccurate mass-to-charge
ratio and migration.
Further, different preparations of genetic material may not migrate
consistently with each other, for morphological or other reasons.
Types of gel
The
types of gel most typically used are agarose and polyacrylamide gels.
Each type of gel is well-suited to different types and sizes of analyte.
Polyacrylamide gels are usually used for proteins, and have very high
resolving power for small fragments of DNA (5-500 bp). Agarose gels on
the other hand have lower resolving power for DNA but have greater
range of separation, and are therefore used for DNA fragments of usually
50-20,000 bp in size, but resolution of over 6 Mb is possible with pulsed field gel electrophoresis (PFGE).
Polyacrylamide gels are run in a vertical configuration while agarose
gels are typically run horizontally in a submarine mode. They also
differ in their casting methodology, as agarose sets thermally, while
polyacrylamide forms in a chemical polymerization reaction.
Agarose
Inserting the gel comb in an agarose gel electrophoresis chamber
Agarose gels are made from the natural polysaccharide polymers extracted from seaweed.
Agarose gels are easily cast and handled compared to other matrices,
because the gel setting is a physical rather than chemical change.
Samples are also easily recovered. After the experiment is finished, the
resulting gel can be stored in a plastic bag in a refrigerator.
Agarose gels do not have a uniform pore size, but are optimal for electrophoresis of proteins that are larger than 200 kDa. Agarose gel electrophoresis can also be used for the separation of DNA fragments ranging from 50 base pair
to several megabases (millions of bases), the largest of which require
specialized apparatus. The distance between DNA bands of different
lengths is influenced by the percent agarose in the gel, with higher
percentages requiring longer run times, sometimes days. Instead high
percentage agarose gels should be run with a pulsed field electrophoresis (PFE), or field inversion electrophoresis.
"Most agarose gels are made with between 0.7% (good separation or
resolution of large 5–10kb DNA fragments) and 2% (good resolution for
small 0.2–1kb fragments) agarose dissolved in electrophoresis buffer. Up
to 3% can be used for separating very tiny fragments but a vertical
polyacrylamide gel is more appropriate in this case. Low percentage gels
are very weak and may break when you try to lift them. High percentage
gels are often brittle and do not set evenly. 1% gels are common for
many applications."
Polyacrylamide
Polyacrylamide gel electrophoresis (PAGE) is used for separating
proteins ranging in size from 5 to 2,000 kDa due to the uniform pore
size provided by the polyacrylamide gel. Pore size is controlled by
modulating the concentrations of acrylamide and bis-acrylamide powder
used in creating a gel. Care must be used when creating this type of
gel, as acrylamide is a potent neurotoxin in its liquid and powdered
forms.
Traditional DNA sequencing techniques such as Maxam-Gilbert or Sanger
methods used polyacrylamide gels to separate DNA fragments differing by
a single base-pair in length so the sequence could be read. Most modern
DNA separation methods now use agarose gels, except for particularly
small DNA fragments. It is currently most often used in the field of immunology and protein analysis, often used to separate different proteins or isoforms of the same protein into separate bands. These can be transferred onto a nitrocellulose or PVDF membrane to be probed with antibodies and corresponding markers, such as in a western blot.
Typically resolving gels
are made in 6%, 8%, 10%, 12% or 15%. Stacking gel (5%) is poured on
top of the resolving gel and a gel comb (which forms the wells and
defines the lanes where proteins, sample buffer and ladders will be
placed) is inserted. The percentage chosen depends on the size of the
protein that one wishes to identify or probe in the sample. The smaller
the known weight, the higher the percentage that should be used. Changes
on the buffer system of the gel can help to further resolve proteins of
very small sizes.
Starch
Partially hydrolysed
potato starch makes for another non-toxic medium for protein
electrophoresis. The gels are slightly more opaque than acrylamide or
agarose. Non-denatured proteins can be separated according to charge and
size. They are visualised using Napthal Black or Amido Black staining.
Typical starch gel concentrations are 5% to 10%.
Gel conditions
Denaturing
TTGE
profiles representing the bifidobacterial diversity of fecal samples
from two healthy volunteers (A and B) before and after AMC (Oral
Amoxicillin-Clavulanic Acid) treatment
Denaturing
gels are run under conditions that disrupt the natural structure of the
analyte, causing it to unfold into a linear chain. Thus, the mobility
of each macromolecule depends only on its linear length and its mass-to-charge ratio. Thus, the secondary, tertiary, and quaternary levels of biomolecular structure are disrupted, leaving only the primary structure to be analyzed.
Nucleic acids are often denatured by including urea in the buffer, while proteins are denatured using sodium dodecyl sulfate, usually as part of the SDS-PAGE process. For full denaturation of proteins, it is also necessary to reduce the covalent disulfide bonds that stabilize their tertiary and quaternary structure, a method called reducing PAGE. Reducing conditions are usually maintained by the addition of beta-mercaptoethanol or dithiothreitol. For general analysis of protein samples, reducing PAGE is the most common form of protein electrophoresis.
Denaturing conditions are necessary for proper estimation of
molecular weight of RNA. RNA is able to form more intramolecular
interactions than DNA which may result in change of its electrophoretic mobility. Urea, DMSO and glyoxal are the most often used denaturing agents to disrupt RNA structure. Originally, highly toxic methylmercury hydroxide was often used in denaturing RNA electrophoresis, but it may be method of choice for some samples.
Denaturing gel electrophoresis is used in the DNA and RNA banding pattern-based methods temperature gradient gel electrophoresis (TGGE) and denaturing gradient gel electrophoresis (DGGE).
Native
Specific enzyme-linked staining: Glucose-6-Phosphate Dehydrogenase isoenzymes in Plasmodium falciparum infected Red blood cells
Native gels are run in non-denaturing conditions, so that the
analyte's natural structure is maintained. This allows the physical
size of the folded or assembled complex to affect the mobility, allowing
for analysis of all four levels of the biomolecular structure. For
biological samples, detergents are used only to the extent that they are
necessary to lyse lipid membranes in the cell.
Complexes remain—for the most part—associated and folded as they would
be in the cell. One downside, however, is that complexes may not
separate cleanly or predictably, as it is difficult to predict how the
molecule's shape and size will affect its mobility. Addressing and
solving this problem is a major aim of quantitative native PAGE.
Unlike denaturing methods, native gel electrophoresis does not use a charged denaturing agent. The molecules being separated (usually proteins or nucleic acids) therefore differ not only in molecular mass
and intrinsic charge, but also the cross-sectional area, and thus
experience different electrophoretic forces dependent on the shape of
the overall structure. For proteins, since they remain in the native
state they may be visualised not only by general protein staining
reagents but also by specific enzyme-linked staining.
A specific experiment example of an application of native gel
electrophoresis is to check for enzymatic activity to verify the
presence of the enzyme in the sample during protein purification. For
example, for the protein alkaline phosphatase, the staining solution is a
mixture of 4-chloro-2-2methylbenzenediazonium salt with
3-phospho-2-naphthoic acid-2’-4’-dimethyl aniline in Tris buffer. This
stain is commercially sold as kit for staining gels. If the protein is
present, the mechanism of the reaction takes place in the following
order: it starts with the de-phosphorylation of 3-phospho-2-naphthoic
acid-2’-4’-dimethyl aniline by alkaline phosphatase (water is needed for
the reaction). The phosphate group is released and replaced by an
alcohol group from water. The electrophile 4- chloro-2-2
methylbenzenediazonium (Fast Red TR Diazonium salt) displaces the
alcohol group forming the final product Red Azo dye. As its name
implies, this is the final visible-red product of the reaction. In
undergraduate academic experimentation of protein purification, the gel
is usually ran next to commercial purified samples in order to visualize
the results and conclude whether or not purification was successful.
Native gel electrophoresis is typically used in proteomics and metallomics. However, native PAGE is also used to scan genes (DNA) for unknown mutations as in Single-strand conformation polymorphism.
Buffers
Buffers
in gel electrophoresis are used to provide ions that carry a current
and to maintain the pH at a relatively constant value.
These buffers have plenty of ions in them, which is necessary for the
passage of electricity through them. Something like distilled water or
benzene contains few ions, which is not ideal for the use in
electrophoresis. There are a number of buffers used for electrophoresis. The most common being, for nucleic acids Tris/Acetate/EDTA (TAE), Tris/Borate/EDTA (TBE). Many other buffers have been proposed, e.g. lithium borate,
which is almost never used, based on Pubmed citations (LB), iso
electric histidine, pK matched goods buffers, etc.; in most cases the
purported rationale is lower current (less heat) matched ion
mobilities, which leads to longer buffer life. Borate is problematic;
Borate can polymerize, or interact with cis diols such as those found in
RNA. TAE has the lowest buffering capacity but provides the best
resolution for larger DNA. This means a lower voltage and more time, but
a better product. LB is relatively new and is ineffective in resolving
fragments larger than 5 kbp; However, with its low conductivity, a much
higher voltage could be used (up to 35 V/cm), which means a shorter
analysis time for routine electrophoresis. As low as one base pair size
difference could be resolved in 3% agarose gel with an extremely low
conductivity medium (1 mM Lithium borate).
Most SDS-PAGE protein separations are performed using a "discontinuous" (or DISC) buffer system
that significantly enhances the sharpness of the bands within the gel.
During electrophoresis in a discontinuous gel system, an ion gradient is
formed in the early stage of electrophoresis that causes all of the
proteins to focus into a single sharp band in a process called isotachophoresis.
Separation of the proteins by size is achieved in the lower,
"resolving" region of the gel. The resolving gel typically has a much
smaller pore size, which leads to a sieving effect that now determines
the electrophoretic mobility of the proteins.
Visualization
After the electrophoresis is complete, the molecules in the gel can be stained to make them visible. DNA may be visualized using ethidium bromide which, when intercalated into DNA, fluoresce under ultraviolet light, while protein may be visualised using silver stain or Coomassie Brilliant Blue
dye. Other methods may also be used to visualize the separation of the
mixture's components on the gel. If the molecules to be separated
contain radioactivity, for example in a DNA sequencing gel, an autoradiogram can be recorded of the gel. Photographs can be taken of gels, often using a Gel Doc system.
Downstream processing
After separation, an additional separation method may then be used, such as isoelectric focusing or SDS-PAGE.
The gel will then be physically cut, and the protein complexes
extracted from each portion separately. Each extract may then be
analysed, such as by peptide mass fingerprinting or de novo peptide sequencing after in-gel digestion. This can provide a great deal of information about the identities of the proteins in a complex.
Applications
- Estimation of the size of DNA molecules following restriction enzyme digestion, e.g. in restriction mapping of cloned DNA.
- Analysis of PCR products, e.g. in molecular genetic diagnosis or genetic fingerprinting
- Separation of restricted genomic DNA prior to Southern transfer, or of RNA prior to Northern transfer.
Gel electrophoresis is used in forensics, molecular biology, genetics, microbiology and biochemistry.
The results can be analyzed quantitatively by visualizing the gel with
UV light and a gel imaging device. The image is recorded with a computer
operated camera, and the intensity of the band or spot of interest is
measured and compared against standard or markers loaded on the same
gel. The measurement and analysis are mostly done with specialized
software.
Depending on the type of analysis being performed, other
techniques are often implemented in conjunction with the results of gel
electrophoresis, providing a wide range of field-specific applications.
Nucleic acids
An agarose gel of a PCR product compared to a DNA ladder.
In the case of nucleic acids, the direction of migration, from
negative to positive electrodes, is due to the naturally occurring
negative charge carried by their sugar-phosphate backbone.
Double-stranded DNA fragments naturally behave as long rods, so
their migration through the gel is relative to their size or, for cyclic
fragments, their radius of gyration. Circular DNA such as plasmids,
however, may show multiple bands, the speed of migration may depend on
whether it is relaxed or supercoiled. Single-stranded DNA or RNA tend
to fold up into molecules with complex shapes and migrate through the
gel in a complicated manner based on their tertiary structure.
Therefore, agents that disrupt the hydrogen bonds, such as sodium hydroxide or formamide, are used to denature the nucleic acids and cause them to behave as long rods again.
Gel electrophoresis of large DNA or RNA is usually done by agarose gel electrophoresis. See the "Chain termination method"
page for an example of a polyacrylamide DNA sequencing gel.
Characterization through ligand interaction of nucleic acids or
fragments may be performed by mobility shift affinity electrophoresis.
Electrophoresis of RNA samples can be used to check for genomic
DNA contamination and also for RNA degradation. RNA from eukaryotic
organisms shows distinct bands of 28s and 18s rRNA, the 28s band being
approximately twice as intense as the 18s band. Degraded RNA has less
sharply defined bands, has a smeared appearance, and intensity ratio is
less than 2:1.
Proteins
SDS-PAGE autoradiography – The indicated proteins are present in different concentrations in the two samples.
Proteins,
unlike nucleic acids, can have varying charges and complex shapes,
therefore they may not migrate into the polyacrylamide gel at similar
rates, or at all, when placing a negative to positive EMF on the sample.
Proteins therefore, are usually denatured in the presence of a detergent such as sodium dodecyl sulfate (SDS) that coats the proteins with a negative charge.
Generally, the amount of SDS bound is relative to the size of the
protein (usually 1.4g SDS per gram of protein), so that the resulting
denatured proteins have an overall negative charge, and all the proteins
have a similar charge-to-mass ratio. Since denatured proteins act like
long rods instead of having a complex tertiary shape, the rate at which
the resulting SDS coated proteins migrate in the gel is relative only to
its size and not its charge or shape.
Proteins are usually analyzed by sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE), by native gel electrophoresis, by preparative gel electrophoresis (QPNC-PAGE), or by 2-D electrophoresis.
Characterization through ligand interaction may be performed by electroblotting or by affinity electrophoresis in agarose or by capillary electrophoresis as for estimation of binding constants and determination of structural features like glycan content through lectin binding.
Nanoparticles
A
novel application for the gel electrophoresis is to separate or
characterize metal or metal oxide nanoparticles (e.g. Au, Ag, ZnO, SiO2)
regarding size, shape or surface chemistry of the nanoparticles. The
scope is to obtain a more homogeneous sample (e.g. narrower particle
size distribution), which than can be used in further products/processes
(e.g. self-assemly processes). For the separation of nanoparticles
within a gel the particle size in relation to the mesh size is the key
parameter, whereby two migration mechanisms where identified: the
unrestricted mechanism, where the particle size << mesh size and
the restricted mechanism, where particle size is similar to mesh size.
History
- 1930s – first reports of the use of sucrose for gel electrophoresis
- 1955 – introduction of starch gels, mediocre separation (Smithies)
- 1959 – introduction of acrylamide gels; disc electrophoresis (Ornstein and Davis); accurate control of parameters such as pore size and stability; and (Raymond and Weintraub)
- 1966 – first use of agar gels
- 1969 – introduction of denaturing agents especially SDS separation of protein subunit (Weber and Osborn)
- 1970 – Laemmli separated 28 components of T4 phage using a stacking gel and SDS
- 1972 – agarose gels with ethidium bromide stain
- 1975 – 2-dimensional gels (O’Farrell); isoelectric focusing then SDS gel electrophoresis
- 1977 – sequencing gels
- 1983 – pulsed field gel electrophoresis enables separation of large DNA molecules
- 1983 – introduction of capillary electrophoresis
- 2004 – introduction of a standardized time of polymerization of acrylamide gels enables clean and predictable separation of native proteins (Kastenholz)
A 1959 book on electrophoresis by Milan Bier cites references from the 1800s. However, Oliver Smithies
made significant contributions. Bier states: "The method of Smithies
... is finding wide application because of its unique separatory power."
Taken in context, Bier clearly implies that Smithies' method is an
improvement.
