HIV-Test, often also called "AIDS-test"
The first test used is an enzyme-linked immunosorbent assay
(ELISA). This is a test to see whether the blood of
a person contains antibodies against the AIDS-Virus HIV. This
test can't detect the virus itself or viral nucleic acid but
it can detect the antibodies, special proteins, which the
immune-system of the infected person has made to fight the
virus. If such antibodies are found, the test is "positive".
In this case, the ELISA is repeated to be sure of the results.
If this second ELISA gives a positive result, another more
sensitive test, called Western blot is done. If the
Western blot is positive, a second blood sample is tested
in a Western blot. Only if all of these tests are positive,
is a person regarded to be "HIV-positive". False-positive
results are extremely rare (about 1 out of every 20 000 tests).
Because the immune-system needs some time to make antibodies
in quantities in which they can be detected this test can't
work immediately after the infection took place. It takes
about 6 to 12 weeks after exposure to the virus to develop
enough antibodies to measure. A person having an HIV-test
during this period might test negative even if he or she is
infected. This is called a false-negative result.
An earlier detection of an HIV-Infection is only possible
through the direct measurement of the viral nucleic acid in
the patient's blood (see "viral load"). But these
tests are much more expensive and not used for routine screening.
How were the modern antiviral drugs developed?
In modern drug research scientists investigate the molecular
mechanisms of a disease and try to find the most promising
targets for drugs. Basic research can be very important, for
example, when scientists searched for the cause of AIDS, which
turned out to be a retrovirus later called HIV, it was very
helpful that they already knew a lot about retroviruses and
their characteristics in general.
After the identification of the HI virus, scientists learned
about it in detail, its components and the specific roles
these components have during the life cycle of the virus in
a human cell. For both the identification of the virus and
the investigation of its molecular structure and function,
many standard procedures of modern biotechnology and gene
technology were used. The virus was studied directly by electron
microscopy Its genome was sequenced, and all its
proteins were characterised and their functions identified.
All this data collected by scientists around the world led
to our understanding of HIV and the mechanisms of its life
cycle in a human cell.
Theoretically, there are many steps in the viral life cycle,
which are possible targets for antiviral drugs. So far the
best targets are two viral enzymes, the "reverse transcriptase"
(RT) and the "protease". The first drug, developed
in 1986, was AZT, a so-called RT inhibitor. The first protease
inhibitor (PI) came on the market in 1996. PIs are very effective
drugs but they can also have serious side effects. All anti-HIV
drugs in use today inhibit these two viral enzymes in various
ways. Attempts to block other viral enzymes or important structures,
e.g. receptor molecules which the virus needs to identify
its target cells, are subject to intense research.
Viral load measurement
Viral load measurement means the direct determination of the
amount of HI viruses in the patient's blood . What is measured
is the quantity of copies of HIV-RNA per ml blood plasma.
The methods used are either based on the direct amplification
of the nucleic acid (i.e. strong, exactly defined multiplication
of the RNA copies in the sample), mainly by PCR, or
on the high amplification of the measured signal (branched
DNA assay, bDNA). Currently, the lower detection limit
is 5 to 20 virus copies per ml plasma, depending on which
method is used. These are quite low numbers; in comparison,
more than 30 000 viral copies per ml plasma would be regarded
as a high viral load. The upper detection limit is about 10
million copies per ml blood plasma.
The viral load is a very reliable marker for the progress
of the infection. Today it is the most important indicator
for the effectiveness of antiretroviral therapy or for the
need to change a current therapy. The aim of the therapy is
the lowest viral load possible - at best an "undetectable"
level of virus copies in the patient's blood.
T-cell count or CD4-cell count
T4 cells or CD4 cells are a special type of white blood cells,
which play an important and central role in the immune system
of the human body. Unfortunately, they are also the favorite
host cells of HI viruses, which attack and destroy them. A
healthy individual has about 800 to 1500 CD4 cells per ml
plasma. If there are less than 200 CD4 cells per microliter
blood, the immune defense becomes incomplete.
Combined with the viral load the CD4-cell count is a reliable
indicator for the patient's condition. The CD4 cells are counted
directly from the blood sample using a method called "laser
flow cytometry". Through the binding of monoclonal antibodies,
which recognize specific surface structures on these cells,
the CD4 cells are labelled with special fluorescent markers.
This allows scientists to distinguish these cells from all
others in the sample and to count them while they are passing
a detector.
Washing sperm
The semen of an HIV-positive man might contain high numbers
of viruses, even under antiretroviral therapy. Luckily, the
viruses do not normally stick to the live sperm cells (which
are needed for impregnation). Instead, they are mainly found
free in the fluid or connected to dead sperm cells and other
cells in the semen. Therefore, it is possible to separate
live sperm cells from the free viruses and infected cells.
Scientists do this through a kind of 'washing' which includes
three steps of careful density gradient centrifugation.
The 'washed' sperm sample is then carefully checked for virus
nucleic acid using highly sensitive detection methods like
PCR. During this procedure, the remaining sperm cells are
stored by cryoconservation to keep them alive. Once it has
been proved that the sperm cells are virus-free (i.e. not
even the slightest trace of virus-DNA or -RNA has been found)
this sperm is used for artificail insemination or IVF.
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