Immunohistochemistry (IHC)
Lab #6:Immunohistochemistry (IHC) Prepared by: El-Hindi.M. &
Abdelmoneim.A. Practical Of Histopathology
20151Objective: Understand Immuonhistochemistry (IHC)
NeurobiotinCalbindinMerged image2
Overview Imunohistochemistry (IHC) combines histological,
immunological and biochemical techniques for the identification of
specific tissue components by means of a specific antigen/antibody
reaction tagged with a visible label.
3Cont. The body's response to the introduction of a foreign
agent, known as the immune response, results in the production of
antibodies which bind the offending material.
Antibodies bind tightly and specifically to an "epitope" (one
specific structure) on an "antigen" (foreign molecule or
structure). 4Fab regionParatope + EpitopeAb-Ag complex5
Theparatopeis the part of an antibody which recognizes an
antigen, the antigen-binding site of an antibody
Anepitope, also known as antigenic determinant, is the part of
an antigen that is recognized by the immune system, specifically by
antibodies, B cells, or T cells.5 Polyclonal Ag injected into host
animal. Serum collected and purified. Multiple antibodies produced
by different cell types bind multiple epitopes on Ag
Monoclonal Ag injected into mouse. Lymphocytes isolated,
hybridized. One antibody produced by one cell type binds one
epitope on Ag.
6Cont. An antigen can be defined as "anything that can be bound
by an antibody."
This can be an enormous range of substances from simple
chemicals, sugars, and small peptides to complex protein complexes
such as a virus capsid.
7Cont. Not all antigens directly elicit an antibody
response.
Some require a carrier to be effective. These generally smaller
antigens are called haptens.
8Haptens are small molecules thatelicit an immune responseonly
when attached to a large carrier such as aprotein; the carrier may
be one that also does not elicit an immune response by
itself.8Cont. Antibodies can be generated by injecting animals with
antigens, and then collecting serum after the immune response has
taken place. If the antibodies are labeled with an easily
detectable molecule (a fluorescent dye, an enzyme, etc.), they
become powerful detection reagents for the antigen.
This system has been exploited to generate exceptionally
specific and sensitive "stains" which are used in histology as well
as other disciplines.
9Cont. The basic process depends upon selecting an antibody
sufficiently specific to bind an antigen in situ.
The antibody/antigen conjugate is then identified using a
variety of signal generating molecules triggered either by the
antibody/antigen interaction or by secondary processes.
The signal generators can be precipitating dyes, fluorescent
molecules or electron dense (ultrastructural tag) materials for
electron microscopy (EM).10
11Cont. Immunohistochemistry is generally carried out in
sectioned tissue, which allows the antibodies free access to the
interior of the cells.
Immunohistochemistry can also be carried out on cells either in
free solution or bound to membranes, or on monolayers of cultured
cells.12Cont. Intracellular Immunohistochemistry requires that the
antibody to the target antigen be able to penetrate the cell
membrane and whatever cell wall may be present before it can attach
to the antigen.
This requires a number of steps not required for sectioned
tissue.13Cont. Primarily the cell membrane must be made permeable
to the antibody, though at the same time the integrity of the cell
contents and structures must be maintained.
This is normally achieved through the use of a specialized
buffer containing a detergent.14
151617Indirect method a fluorescent labeled antibody is prepared
against the primary antibody specific for the macromolecule of
interest.
forming a secondary complex visible by fluorescent
microscopy
1819
Cont.The indirect method is more sensitive than the direct
method because numerous labeled anti-antibodies bind to the primary
antibody, making them easier to visualize.
In addition, the indirect method does not require labeling of
the primary antibody, which often is available only in limited
quantities.
20Cont.Immunocytochemistry can be used with specimens for
electron microscopy by labeling the antibody with ferritin, an
electron-dense molecule, instead of with a fluorescent dye.
Ferritin labeling can be applied in both the direct and indirect
methods.21
22General Immunohistochemistry Protocol23Part 11. Fixation Fresh
unfixed, fixed, or formalin fixation and paraffin embedding2.
Sectioning 3. Whole Mount Preparation
Tissue preparation 2424Part 21. Antigen retrieval Proteolytic
enzyme method and Heat-induced method2. Inhibition of endogenous
tissue components 3% H2O2, 0.01% avidin3. Blocking of nonspecific
sites 10% normal serum pretreatment2525Part 3Make a selection based
on the type of specimen, the primary antibody, the degree of
sensitivity and the processing time required.staining2626Positive
Control It is to test for a protocol or procedure used. It will be
ideal to use the tissue of known positive as a control. Negative
Control It is to test for the specificity of the antibody involved.
Controls 2727
2828
2929What cellular antigens can we target?CytoplasmicNuclearCell
membraneLipidsProteins
30Identify replicating cells
31Locate cells that are signaling
32Locate apoptotic cells
33Identify activation states
34Identify different types of cells in a tissue
35Examine cytoskeletal structure
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