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So you've sent your swab back to us. What happens next? Read
on to see the processes your sample goes through to get your
set of numbers that allows you to compare yourself with your
relatives and thousands others worldwide.
 Laboratory
Preparation
Workflow is always unidirectional from DNA Extraction through
to Detection which ensures that cross-contamination of DNA
samples doesn't occur. This includes specimens, reagents,
and paperwork.
Every laboratory work surface is disinfected with 10% bleach
in water followed by a 100% ethanol rinse at least once per
day. This removes any traces of contamination from the surface.
General protocols require that all surfaces and equipment
are cleaned at least once per day as well as before and after
any operation or process setup.
To assure that there are undetectable levels of contamination,
at least once per week two separate surfaces in the Extraction
or PCR Setup areas are wipe tested to check for the presence
of amplified DNA.
DNA
Extraction
When a sample comes in, the bar-coded sample number is utilised
to allow tracking of the sample at every stage. Each test
is run in duplicate and the results married up at the end
to ensure consistent results.
Before we can test the DNA, we have to extract it from the
chromosomes from within the cells. We do this using a series
of extractions.
Most extractions (i.e., swab specimens) are performed on our
QIAGEN BioRobot 8000, which can extract 4 plates of 96 samples
and controls (a total of 384 samples) at one time, simultaneously.
Each extraction batch includes quality controls to monitor
for, and detect possibilities of contamination. This ensures
reagent quality and the specificity of the test.
All reagents for PCR are prepared in a dedicated dead air
box, under low light conditions, and on ice to ensure contamination
free master mix and optimum sensitivity for all fluorescent
labels.
Extracted DNA, master mix, and controls are automatically
combined and loaded onto 384 well plates.
Amplification
After PCR setup, the plates are transferred into the Amplification
Laboratory through a dedicated one way pass-through box on
the wall of the laboratory. This pass through box helps to
minimize contamination and maintain unidirectional work flow
into the amplification area.
The laboratory utilizes several ABI 9700 thermo cyclers.
These are all networked into a central computer that serves
the specific amplification protocols dependent on the test
type and markers being amplified. Our Laboratory Information
System (LIMS) records and tracks which machine and protocol
is run for each plate.
Detection
After amplification, the amplified DNA is combined with formamide
and size standard on our second Biomek FX robot. Formamide
is a chemical that denatures the DNA amplicon and facilitates
detection and electrophoresis. The size standard is called
the 'Ladder' which ensures that each allele is correctly located
in the associated bin for its specific fragment size.
The plate is quickly heated to 96 ºC for several minutes
to facilitate the denaturation and then placed in the freezer
for several minutes to 'freeze' in the denatured DNA.
The plate is then loaded onto any of our several ABI detection
machines. We use a combination of machines for different purposes.
We use an ABI 3100 for basic research and panel development.
We use our ABI 3700's for high-throughput sequencing and finally
we use our several ABI 3730's for high-throughput fragment
analysis work.
Once the plate has been run through analysis it is placed
in the Detection refrigerator for short term storage to ensure
that the run passes all Quality Control checks.
Analysis
Our laboratory tracking system automatically uploads the
data files from the detection instruments and launches GeneScan
and GenoTyper software programs. These programs are used to
assess the quality of each run and sample as well as to assign
the specific alleles to each fragment analyzed.
Each sample in each batch run through Detection is analyzed
and called by two independent analysts. Their calls are compared
by the laboratory information system and any discrepancies
are brought out for resolution by our lead analyst.
Since each swab specimen is extracted in duplicate, there
are two distinct batches for each sample that comes off the
detection instruments. This results in 4 separate readings
of each marker for each person we test. If any discrepancy
results then the sample may be recollected or the third swab
extracted.
Quality
Control
The following controls are used on every batch and plate
processed, and is reviewed at the Analysis step:
- Negative Extraction. This is basically a check to ensure
that the extraction reagents are clean and that no amplification
occurs. If any peaks come up in this control the whole batch
fails and is re-extracted.
- PCR Negative Control. Like the extraction negative control
we ensure that the reagents and master mix for PCR are clean
and do not give rise to spurious peaks.
- PCR Positive Control(s). One or more controls are added
to each plate to ensure that the correct calls are being made
for each plate. Positive controls use a combination of NIST
SRM, CEPH DNA, and employee DNA samples. These controls allow
for us to ensure that each plate runs correctly, that it gives
the correct results without shifting data, and allows for
an assessment of contamination control.
- DNA Ladders. Each sample's alleles line up within specified
bins defined by the size standard or ladder each was processed
with. A QC check is performed to ensure that each allele is
within the expected bin location.
- Data matching between analysts and batches. The analysts
ensure consistency between the two batches and the two independent
reviews. This makes a total of 4 unique readings and reviews
of each person's genotype.
Reporting
The lead analyst prints out the final report for the individual
being reported. A clerical/administrative review of the case
file and report is conducted to ensure that all is in order
and that no typographic errors have been entered into the
laboratory tracking system.
The final report is then reviewed by either the Laboratory
Supervisor, Laboratory Manager, or the Laboratory Director,
depending on the type of case.
Once all reviews are conducted the report is signed by the
final reviewer(s) and uploaded to Oracle and released.
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