Western Blotting
Western Blotting
Western Blotting
IMMUNOLOG
Y
INTRODUCTION
The western blot (sometimes called the protein immunoblot) is a widely used analytical
technique in molecular biology used to detect specific proteins in the given sample or mixture
of proteins. It involves gel electrophoresis to separate out native proteins by 3-D structure or
denatured proteins by the length of the polypeptide. Then proteins are then transferred to a
membrane (typically nitrocellulose or PVDF), where they are stained with antibodies specific
to the target protein. There are currently many reagent synthesizing companies that specialize
in providing antibodies (both monoclonal and polyclonal antibodies) against tens of thousands
of different proteins. This method is used in the fields of molecular biology, biochemistry,
immunogenetics and other molecular biology disciplines. The method originated in the
laboratory of Harry Towbin at the Friedrich Miescher Institute. The name western blot was
given to the technique by W. Neal Burnette and is a play on the name Southern blot, a
technique for DNA detection developed earlier by Edwin Southern. Detection of RNA is
termed northern blot and was developed by George Stark at Stanford. A general outline of
western blotting is as follows:
STEPS OF WESTERN BLOT
Tissue Preparation
Samples should be taken from whole tissue or from cell culture. Solid tissues are initially
disintegrated mechanically using a blender (for larger sample volumes), using a homogenizer
(smaller volumes), or by the process of sonication. However, virus or environmental samples
are also the source of protein and thus western blotting is also used to study them. Assorted
detergents, salts, and buffers may be involved to aid in the lysis of cells and to solubilize
proteins. Protease and phosphatase inhibitors are often used to avoid the digestion of the
sample by its self-enzymes. Tissue preparation is done at very low temperatures to avoid
protein conformational alterations- denaturing and degradation. A blend of biochemical and
mechanical processes – involving various types of filtration and centrifugation – can be
incorporated to separate different cellular organelles.
Gel Electrophoresis
The proteins of the sample used are separated using the technique of gel electrophoresis.
Separation of proteins may be on the basis of molecular weight, isoelectric point (pI), electric
charge, or a combination of these parameters. The condition of the separation is dependent on
the treatment of the sample and the condition of the gel. This is an important technique to
identify a protein.
The most common type of gel electrophoresis involves polyacrylamide gels and buffers filled
with sodium dodecyl sulfate (SDS). SDS-PAGE (SDS polyacrylamide gel electrophoresis)
stabilizes polypeptides in a denatured condition once they have been treated with reducing
agents to remove secondary and tertiary structure (e.g. disulfide bonds [S-S] to sulfhydryl
groups [SH and SH]) and thus gives separation of proteins on the basis of their molecular
weight. Sampled proteins got loaded in the negatively charged SDS and approach to the
positively charged electrode through the acrylamide mesh of the gel. Smaller proteins move
faster through this mesh and the proteins are thus separated according to size (usually measured
in kilodaltons, kDa). The concentration of acrylamide used determines the resolution of the gel
- the greater the concentration the better the resolution of lower molecular weight proteins. The
lower the acrylamide concentration the better the resolution of higher molecular weight
proteins. Proteins travel only in one direction along the gel for most blots. Samples are
carefully loaded into wells in the gel. One lane is usually reserved for a marker or ladder, a
commercially available mixture of proteins having defined molecular weights, typically stained
so as to form visible, colored bands. When DC voltage is applied along the gel, proteins start
moving through it at different speeds dependent on molecular weight. These different rates of
migrations (different electrophoretic mobilities) separate into bands within each lane. It is also
possible to involve a two-dimensional (2-D) gel which spreads the proteins from a single
sample out in two dimensions. Proteins got separated according to their isoelectric point (pH at
which they have neutral net charge) in the one dimension, and according to their molecular
weight
Detection
During the detection step the membrane is "probed" for the protein of interest with a modified
antibody which is conjugated to a reporter enzyme; when exposed to an appropriate substrate
this enzyme gives a colorimetric reaction and gives a color. For a variety of reasons, this
traditionally takes place in a two-step process, although there are now one-step detection
methods available for certain applications.
Two Steps
Primary Antibody
The primary antibodies are produced when a host species or immune cell culture is exposed to
protein of interest (or a part thereof). Normally, this is an event of the immune response,
whereas here they are harvested and involved in sensitive and specific detection, that attach the
protein directly. After blocking, a dilute solution of primary antibody (generally between 0.5
and 5 micrograms/mL) is incubated with the membrane under gentle agitation. Generally, the
solution is composed of buffered saline solution with a small percentage of detergent, and
sometimes with powdered milk or BSA. The antibody solution and the membrane can be sealed
and incubated together for anywhere from 30 minutes to overnight. It can also be incubated at
different temperatures, with warmer temperatures being associated with more binding, both
specific (to the target protein, the "signal") and non-specific ("noise").
Secondary Antibody
After rinsing the membrane to remove unbound primary antibody, the membrane is exposed
to another antibody, directed at a species-specific portion of the primary antibody.
Antibodies come from animal sources (or animal sourced hybridoma cultures); an anti-
mouse secondary will bind to almost any mouse-sourced primary antibody, which allows
some cost savings by allowing an entire lab to share a single source of mass-produced
antibody, and provides far more consistent results. This is known as a secondary antibody,
and due to its targeting properties, tends to be referred to as "anti-mouse," "anti-goat," etc.
The secondary antibody is usually linked to biotin or to a reporter enzyme such as alkaline
phosphatase or horseradish peroxidase. This means that several secondary antibodies will
bind to one primary antibody and enhance the signal.
Most commonly, a horseradish peroxidase-linked secondary is used to cleave a
chemiluminescent agent, and the reaction product produces luminescence in proportion to
the amount of protein. A sensitive sheet of photographic film is placed against the
membrane, and exposure to the light from the reaction creates an image of the antibodies
bound to the blot. A cheaper but less sensitive approach utilizes a 4-chloronaphthol stain
with 1% hydrogen peroxide; reaction of peroxide radicals with 4-chloronaphthol produces
a dark purple stain that can be photographed without using specialized photographic film.
As with the ELISPOT and ELISA procedures, the enzyme can be provided with a substrate
molecule that will be converted by the enzyme to a colored reaction product that will be visible on
the membrane (see the figure below with blue bands).
Analysis
After the unbound probes are washed away, the western blot is ready for detection of the
probes that are labeled and bound to the protein of interest. In practical terms, not all
westerns reveal protein only at one band in a membrane. Size approximations are taken by
comparing the stained bands to that of the marker or ladder loaded during electrophoresis.
The process is repeated for a structural protein, such as actin or tubulin, that should not
change between samples. The amount of target protein is normalized to the structural
protein to control between groups. This practice ensures correction for the amount of total
protein on the membrane in case of errors or incomplete transfers.
Radioactive Detection
Radioactive labels do not require enzyme substrates, but rather allow the placement of medical
X- ray film directly against the western blot which develops as it is exposed to the label and
creates dark regions which correspond to the protein bands of interest (see image to the right).
The importance of radioactive detections methods is declining due to its hazardous radiation,
because it is very expensive, health and safety risks are high, and ECL (enhanced
chemiluminescence) provides a useful alternative.Colorimetric Detection, Chemiluminescent
Detection are also used.
Secondary probing
One major difference between nitrocellulose and PVDF membranes relates to the ability
of each to support "stripping" antibodies off and reusing the membrane for subsequent
antibody probes. While there are well-established protocols available for stripping
nitrocellulose membranes, the sturdier PVDF allows for easier stripping, and for more reuse
before background noise limits experiments. Another difference is that, unlike
nitrocellulose, PVDF must be soaked in 95% ethanol, isopropanol or methanol before use.
PVDF membranes also tend to be thicker and more resistant to damage during use.
Troubleshooting
Even though the procedure for western blot is simple, many problems can arise, leading to
unexpected results. The problem can be grouped into five categories:
(1) unusual or unexpected bands, (2) no bands, (3) faint bands or weak signal, (4) high background
on the blot, and (5) patchy or uneven spots on the blot.
Unusual or unexpected bands can be due to protease degradation, which produces bands at
unexpected positions. In this case it is advisable to use a fresh sample which had been kept on
ice or alter the antibody. If the protein seems to be in too high of a position, then reheating the
sample can help to break the quaternary protein structure. Similarly, blurry bands are often
caused by high voltage or air bubbles present during transfer. In this case, it should be ensured
that the gel is run at a lower voltage, and that the transfer sandwich is prepared properly. In
addition, changing the running buffer can also help the problem. Non flat bands can be the result
of too fast of a travel through the gel, due to low resistance. To fix this the gel should be
optimized to fit the sample. Finally, white (negative) bands on the film are due to too much
protein or antibody.
Another problem: no bands can also arise due to many reasons related to antibody, antigen, or buffer
used. If an improper antibody is used, either primary or secondary, the band will not show. In
addition, the concentration of the antibody should be appropriate as well; if the concentration is too
low, the signal may not be visible. It is important to remember that some antibodies are not to be
used for western blot. Another reason for no visible bands is the lowest concentration or absence of
the antigen. In this case, antigen from another source can be used to confirm whether the problem
lies with the sample or with other elements, such as the antibody. Moreover, prolonged washing can
also decrease the signal. Buffers can also contribute to the problem. It should be ensured that buffers
like the transfer buffer, TBST, running buffer and ECL are all new and noncontaminated. If the
buffers are contaminated with sodium azide, it can inactivate HRP.
Similarly, weak signals can be caused by low concentration of antibody or antigen. Increasing
exposure time can also help to make the band clearer. Another reason could be nonfat dry milk
masking the antigen. In this case use BSA or decrease the amount of milk used.
REFERENCES