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Animal
Cell Technology: Becoming more and more
important
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By
definition animal cell technology is that part of
biotechnology which is based on the use of animal
(including human) cells, propagated in vitro, for
the manufacture of biopharmaceuticals and as
toolbox in the discovery and testing of medicines.
The main field of application of animal cell
technology is the medical and pharmaceutical arena.
The members of ACTIP, the Animal Cell Technology
Industrial Platform, want to support and reinforce
further development of animal cell technology which
will lead to increased utilization of animal and
human cells to be propagated in vitro.
As
early as the 19th century, animal cell technology
already formed the basis for providing vaccines
against small pox and rabies, although these
vaccines were actually produced in living animals.
In the 20th century, knowledge in many areas of the
life sciences increased tremendously. In the early
1950s this led to the Salk and Sabin processes of
in vitro cultivation of cells for the production of
highly effective vaccines against polio virus.
Other vaccines against a wide variety of human and
animal viral diseases like rubella, measles, foot
and mouth disease etc. followed soon after. In
addition, novel animal cell technologies made it
possible to develop high throughput assays for the
screening of new candidate pharmaceuticals and as
diagnostic tools.
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Breakthroughs in the 1970s and 1980s
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A
major breakthrough in the field of animal cell
technology came in the late 1970s/early 1980s with
the development of hybridoma and recombinant DNA
technology. The hybridoma technology makes it
possible to elicit, select and produce, in vitro,
so called monoclonal antibodies of consistent
quality, high specificity and unlimited quantities,
whereas previously antibodies could only be
produced in life animals with a varying degree of
quality. Antibodies are nowadays widely used for
passive immunization of patients against infectious
diseases, for diagnostic purposes like blood group
typing and disease testing, and for therapeutic
intervention.
The
development of recombinant DNA technology or
heterogenous gene expression allows for e.g. the
production of human proteins in animal cells at a
relatively efficient production scale. Previously,
many of these human proteins could not be produced
or isolated at all.
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Need
for animal cells
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The
recombinant DNA technology - also called genetic
engineering - makes it possible to transfer a gene
from one species into cells of another, and to let
these transformed cells produce the encoded gene
product. For example, the encoding gene for human
insulin has been successfully transfected into the
easy to grow bacterium Escherichia coli. However,
with more complex and larger gene products than
insulin, it is no longer possible to use bacteria
like E. coli as host cells for the production. The
reason is that these bacteria can not perform the
complicated posttranslational processing steps such
as glycosylation, folding and trimming, which is
often a prerequisite to exert biological functions.
Alternatively, such proteins can be expressed
successfully and correctly in cultured animal
cells. For example, the bioactivity of
erythropoietin, tissue plasminogen activator or
factor VIII is strongly dependent on a correct
posttranslational processing. Development of novel
cell lines has resulted in an increased frequency
in which animal cells are being used. In the early
eighties the majority of biopharmaceuticals was
produced in E. coli (86%), whereas in the early
nineties this figure had been dropped to around
40%, the other 50-60% was produced in animal cells
such as Chinese Hamster Ovary (CHO) cells and Baby
Hamster Kidney (BHK) cells.
Nevertheless,
using animal cells as production factories,
however, has the disadvantage that the production
costs are relatively high in comparison with
production in cultivated bacteria or yeast cells,
and related to this, the relatively small
production scale. Therefore, many research programs
have been and are being started to develop robust
and high-producing animal host cell
lines.
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Therapeutics:
demand for large scale manufacturing
facilities
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At
present, the majority of therapeutic
biopharmaceuticals has been produced using animal
cell technology and include proteins used for the
treatment of cardiovascular diseases (tissue
plasminogen activator: tPA, reteplase), cystic
fibrosis (DNases), anemia (erythropoietin: EPO),
haemophilia (coagulation factors VIII and IX),
cancer and viral infections (interferons and
interleukins), multiple sclerosis
(interferon-beta2) and dwarfism (human growth
hormone: hGH). Monoclonal antibodies are used for
the treatment of a rapidly expanding list of
diseases, e.g. to reduce the rejection of
transplanted organs by the recipient (e.g. Simulect
and Zenapax), to treat metastasized breast cancer
(Herceptin), to treat non-Hodgkin lymphoma's
(Rituxan), to inhibit allergic asthma (Xolair), and
many others (see monograph on monoclonal
antibodies). These different antibody indications
have in common that effective patient dosing
requires relatively large amounts of
antibody-protein, which translates into a huge
demand for large scale manufacturing capacity.
Although only 10% of all biopharmaceuticals relate
to monoclonal antibodies, more than 75% of the
world wide manufacturing capacity is dedicated to
its production. Therefore, improvement of
production processes remains imperative.
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Gene
therapy
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Culturing
of animal cells forms also an important basis for
the new area of gene therapy. In contrast to direct
treatment of patients with recombinant
biopharmaceuticals, gene therapy is based on the
delivery of the corresponding gene to a patient, in
such a way that the patient may produce the
functional gene product (i.e. the protein)
intracellularly. In principle, such an approach is
considered to result in long-lasting treatment or
cure. For the delivery of relevant genes into
specific tissues in patients recombinant viruses
are being used. These viruses are genetically
modified and produced in vitro in animal cells.
Gene therapy is very promising since it may yield a
number of advantages. When we consider for example
patients suffering from a bleeding disorder such as
Haemophilia A, these patients have a deficient gene
encoding for clotting Factor VIII. Current
treatment is based on the life long treatment with
the recombinant protein Factor VIII. Gene therapy
might make it possible to administer the gene
encoding Factor VIII into the liver cells of these
patients. These cells are the natural producer
cells of Factor VIII and, thus, may behave
naturally after transfection with the functional
gene encoding Factor VIII.
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Drug
discovery
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The
evolution of the drug discovery and development
process has been revolutionized by the
implementation of high-throughput technologies,
combinatorial chemistry and genomics-based target
identification and validation. Animal and human
cells have become an essential part of the
cell-based assays and models, which form the basis
of target identification and validation
experiments, HT-screening of chemical libraries for
lead finding and optimization purposes and
HT-testing for ADME/tox of candidate drugs. Given
the fact that these areas are still in rapid
development, it will be obvious that improvement of
cell culture procedures remains a prerequisite. In
this respect, multidisciplinary R&D programmes
remain crucial to feed further progress in the tool
box needed for efficient drug discovery.
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How
are animal cells propagated?
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Animal cells are cultivated in
vitro by mimicking the same conditions as they have
in their natural environment, the body. They need
complex and balanced culture media which contain
substrates such as glucose, amino acids, vitamins,
salts, trace elements and others. Small scale
cultures are performed in tissue culture flasks or
roller bottles in a 37°C incubator.
Large scale cultivation for
industrial purposes is mainly performed in
bioreactors which are large stainless steel tanks
with gentle agitation and aeration to supply
oxygen. In these systems, cells grow, multiply and,
in the case of recombinant cells, release human
proteins into the culture medium from which the
protein product can be purified, formulated and
packaged. Currently, a major development is to
design large scale cultivation procedures utilizing
media free of serum additives or protein growth
factors. Resulting protein free media or procedures
are considered to be far more safe as to the
transfer of biological contamination. Particularly,
potential contamination of biopharmaceutical end
products with agents that may transfer Bovine
Spongiform Encephalitis (BSE) has been the major
driver to develop such protein/serum free media and
related cell culturing processes.
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