'Monoclonal antibodies' ('mAb' or 'moAb') are
antibodies that are identical because they were produced by one type of
immune cell and are all
clones of a single parent cell. Given (almost) any substance, it is possible to create monoclonal antibodies that specifically bind to that substance; they can then serve to detect or purify that substance. This has become an important tool in
biochemistry,
molecular biology and
medicine. When used as medications, the generic name ends in ''-mab'' (see "
Nomenclature of monoclonal antibodies").
Discovery
The idea of a "
magic bullet" was first proposed by
Paul Ehrlich who at the beginning of the 20th century postulated that if a compound could be made that selectively targeted a disease-causing organism, then a toxin for that organism could be delivered along with the agent of selectivity.
In the
1970s the B-cell cancer
myeloma was known, and it was understood that these cancerous B-cells all produce a single type of antibody (a
paraprotein). This was used to study the structure of antibodies, but it was not yet possible to produce identical antibodies specific to a given antigen.
The process of producing monoclonal antibodies described above was invented by
Georges Köhler,
César Milstein, and
Niels Kaj Jerne in
1975;
[1] they shared the
Nobel Prize in Physiology or Medicine in
1984 for the discovery.
The key idea was to use a line of myeloma cells that had lost their ability to secrete antibodies, come up with a technique to fuse these cells with healthy antibody producing B-cells, and be able to select for the successfully fused cells.
In 1988
Greg Winter and his team pioneered the techniques to humanize monoclonal antibodies,
[2] removing the reactions that many monoclonal antibodies caused in some patients.
Production
Researchers looking at slides of cultures of cells that make monoclonal antibodies. These are grown in a lab and the researchers are analyzing the products to select the most promising of them.
Monoclonal antibodies can be grown in unlimited quantities in the bottles shown in this picture.
Technician's hand filling wells with a liquid for a research test. This test involves preparation of cultures in which hybrids are grown in large quantities to produce desired antibody. This is effected by fusing
myeloma cell and
mouse lymphocyte to form a hybrid cell (
hybridoma).
Lab technician bathing prepared slides in a solution. This technician is involved in the preparation of slides of monoclonal antibodies for researchers. These highly specific cells shown are those labeling human
breast cancer.
Hybridoma
Monoclonal antibodies can be produced in
cell culture or in live animals. If a foreign substance (an
antigen) is injected into a
vertebrate such as a
mouse or a
human, some of the
immune system's
B-cells will turn into
plasma cells and start to produce antibodies that recognize that antigen. Each B-cell produces only one kind of antibody, but different B-cells will produce structurally different antibodies that bind to different parts ("
epitopes") of the antigen. This natural mixture of antibodies found in serum is known as
polyclonal antibodies.
To produce ''monoclonal'' antibodies, the B-cells from the
spleen or
lymph nodes are removed from an animal that has been challenged several times with the antigen of interest. These B-cells are then fused with
myeloma tumor cells that can grow indefinitely in culture (myeloma is a B-cell cancer or more specifically a
plasmacytoma) and that have lost the ability to produce antibodies. This fusion is done by making the
cell membranes more permeable by the use of
polyethylene glycol (PEG),
electroporation or, of historical importance, infection with some virus. The fused hybrid cells (called
hybridomas), being cancer cells, will multiply rapidly and indefinitely. Large amounts of antibodies can therefore be produced. The hybridomas are sufficiently diluted to ensure clonality (all cells in the culture stem from the same single cell) and grown. The antibodies from the different clones are then tested for their ability to bind to the antigen (for example with a test such as
ELISA or Antigen Microarray Assay) or immuno-
dot blot, and the most sensitive one is picked out. When the hybridoma cells are injected in
mice (in the
peritoneal cavity, the gut), they produce tumors containing an antibody-rich fluid called
ascites fluid.
In the above process, myeloma cell lines that have lost their ability to produce their own antibodies or antibody chain are used, so as to not contaminate the target antibody. Furthermore, only myeloma cells that have lost a specific
enzyme called
hypoxanthine-guanine phosphoribosyltransferase (HGPRT) and therefore cannot grow under certain conditions (e.g. in the presence of a selection medium called
HAT medium) are used; these cells are preselected by the use of either
8-azaguanine or
6-thioguanine(8-azaguanine has been shown to produce unreliable results.(van Diggelen et al 1979)) media prior to the fusion since cells that possess the HGPRT will be killed by the 8-azaguanine. During the fusion process many cells can fuse: Myeloma cell with myeloma cell, spleen cell with spleen cell, spleen cell with myeloma cell, etc. The desired fusions for making hybridomas are between a healthy B-cell, which produces antibodies against the antigen of interest, and a myeloma cell. In these relatively rare fusions, the healthy B cell will make the HGPRT enzyme that will allow the fused cell to survive in HAT medium so that only the successfully fused cells will grow in culture. The medium must be enriched during selection to favour hybridoma growth. This can be achieved by the use of a layer of feeder cells or supplement media such as
briclone. Production in cell culture is usually preferred as the ascites technique may be very painful to the animal and if replacement techniques exist, may be considered unethical.
Recombinant
The production of
Recombinant monoclonal antibodies involves technologies, referred to as ''repertoire
cloning'' or ''
phage display/
yeast display''. Recombinant antibody engineering involves the use of
viruses or
yeast to create antibodies, rather than mice. These techniques rely on rapid cloning of immunoglobulin gene segments to create libraries of antibodies with slightly different
amino acid sequences from which antibodies with desired specificities can be selected.
[3] These techniques can be used to enhance: the specificity with which antibodies recognize antigens, their stability in various environmental conditions, their therapeutic efficacy, and their detectability in diagnostic applications.
[4] Fermentation chambers have been used to produce these antibodies on a large scale.
Applications
Once monoclonal antibodies for a given substance have been produced, they can be used to detect the presence and quantity of this substance, for instance in a
Western blot test (to detect a protein on a membrane) or an
immunofluorescence test (to detect a substance in a cell). They are also very useful in immunohistochemistry which detect antigen in fixed tissue sections. Monoclonal antibodies can also be used to purify a substance with techniques called
immunoprecipitation and
affinity chromatography.
Monoclonal antibodies for cancer treatment
Main articles: Monoclonal antibody therapy
One possible treatment for
cancer involves monoclonal antibodies that bind only to cancer cell-specific
antigens and induce an immunological response against the target cancer cell. Such mAb could also be modified for delivery of a
toxin,
radioisotope,
cytokine or other active conjugate; it is also possible to design
bispecific antibodies that can bind with their Fab regions both to target antigen and to a conjugate or effector cell. In fact, every intact antibody can bind to cell receptors or other proteins with its Fc region. The illustration below shows all these possibilities:
'Monoclonal antibodies for cancer.'
ADEPT, antibody directed enzyme prodrug therapy; ADCC, antibody dependent cell-mediated cytotoxicity; CDC, complement dependent cytotoxicity; MAb, monoclonal antibody; scFv, single-chain Fv fragment.
[5] Chimeric and humanized antibodies
Main articles: humanized antibodies
One problem in medical applications is that the standard procedure of producing monoclonal antibodies yields mouse antibodies. Although murine antibodies are very similar to human ones there are differences. The human
immune system hence recognizes mouse antibodies as foreign, rapidly removing them from circulation and causing systemic inflammatory effects.
A solution to this problem would be to generate human antibodies directly from humans. However, this is not easy, primarily because it is generally not seen as ethical to challenge humans with antigen in order to produce antibody; while the ethics of doing the same to non-humans is a matter of debate. Furthermore, it is not easy to generate human antibodies against human tissues.
Various approaches using recombinant DNA technology to overcome this problem have been tried since the late 1980s. In one approach, one takes the DNA that encodes the binding portion of monoclonal mouse antibodies and merges it with human antibody producing DNA. One then uses
mammalian
cell cultures to express this DNA and produce these half-mouse and half-human antibodies. (Bacteria cannot be used for this purpose, since they cannot produce this kind of
glycoprotein.) Depending on how big a part of the mouse antibody is used, one talks about 'chimeric antibodies' or 'humanized antibodies'.
Another approach involves mice
genetically engineered to produce more human-like antibodies. Monoclonal antibodies have been generated and approved to treat:
cancer,
cardiovascular disease,
inflammatory diseases,
macular degeneration,
transplant rejection,
multiple sclerosis, and
viral infection (see
monoclonal antibody therapy).
In August 2006 the
Pharmaceutical Research and Manufacturers of America reported that U.S. companies had 160 different monoclonal antibodies in clinical trials or awaiting approval by the
Food and Drug Administration.
[6]
See also
★
Monoclonal antibody therapy
★
Nomenclature of monoclonal antibodies
★
Polyclonal antibody
★
Nanobodies
References
1. Kohler G, Milstein C. ''Continuous cultures of fused cells secreting antibody of predefined specificity.'' Nature 1975;256:495-7. PMID 1172191. Reproduced in J Immunol 2005;174:2453-5. PMID 15728446.
2. Riechmann L, Clark M, Waldmann H, Winter G. ''Reshaping human antibodies for therapy.'' Nature 1988;332:323-7. PMID 3127726.
3. Recombinant monoclonal antibody technology, Siegel DL, , , Transfusion clinique et biologique : journal de la Société française de transfusion sanguine, 2002
4. Phage display: a molecular tool for the generation of antibodies--a review, Schmitz U, Versmold A, Kaufmann P, Frank HG, , , Placenta, 2000
5. Modified from Carter P: Improving the efficacy of antibody-based cancer therapies. Nat Rev Cancer 2001;1:118-129
6. ''PhRMA Reports Identifies More than 400 Biotech Drugs in Development.'' Pharmaceutical Technology, August 24, 2006. Retrieved 2006-09-04.
External links
★
Monoclonal Antibodies, from John W. Kimball's online biology textbook
★
العربية
中国
Français
Deutsch
Ελληνική
हिन्दी
Italiano
日本語
Português
Русский
Español
