Sex-Determination of the Domestic Chicken
(Gallus Gallus)
Abstract
DNA was extracted from three sample types, destructive tissue
sampling, invasive blood sampling and non-invasive feather sampling to
determine the quality and quantity of DNA yields between the three types.
DNA was then used to determine the sex of each sample.
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Introduction
When working with wild animals it is often hard to collect
and extract DNA therefore, non-invasive methods of collection are required. DNA
extraction from animals fall into three categories which are destructive,
non-destructive (invasive) and non-invasive. Destructive sampling requires the
organism to be killed to be able to obtain the tissues necessary for genetic
analysis. This technique is often used when identifying specific enzymes or
metabolic requirements. Non-destructive
or invasive sampling requires capture of the organism in order to take a tissue
biopsy or blood sample. Non-invasive techniques are the most comfortable and
humane way for the animal’s DNA to be extracted and the technique is beneficial
when the organism is endangered or hard to capture. Non-invasive sampling does
not disturb the animal’s habitat and often DNA that has been left behind in
nests such as feathers, skins, bones, eggshells, scats and swabs etc. can be
used. Limitations to non-invasive methods have shown that DNA samples degrade
overtime which becomes troublesome in analysis. Studies have also shown the
amount of DNA extracted is much lower than invasive or destructive means of DNA
extraction therefore more research is required to improve the current
techniques to increase extracted DNA quality.
Good quality DNA visualisation is a key point to determining
whether an experiment was successful or requires more research therefore it is
important to reduce variables that may affect results. During DNA extraction the
quality of DNA may be affected by the technique used for extraction, ensuring
an uncontaminated workspace is available, how the DNA was preserved and the
time period between extraction and use as DNA as it degrades over time.
Storage of DNA is an important factor to ensure the results
are conclusive. Freeland (2005) discusses various methods of preservation which
are available including expensive freezing with liquid nitrogen or dry ice, use
of a deep freezer (<-80°C) or a fridge, or keeping the DNA at room temperature.
These later methods have shown that extracted DNA degrades quicker than liquid
nitrogen freezing but may be useful when extracting DNA in the field. For
optimal results it is best that the time between extraction and analysis is
kept to a minimum. Another method of preservation which is useful in the field
is the use of ethanol which is useful for DNA preservation when a lab is not
available. Colton and Clark (2001) tested various storage conditions over a 21
month period showing the importance of freezing the samples, preferably in
ethanol. Freezing the DNA samples at -20°C were used during our experiment
therefore DNA degradation was not a variable factor between the samples.
Different DNA extraction and analysis methods use varying
chemicals, reagents, buffers, salts or commercial kits therefore to reduce
variables it is crucial to check the use by dates throughout the procedure as
reagents that have been sitting around for long periods of time affect pH,
chemical bonding and structures giving you inconclusive results or lower
quality DNA samples.
Good quality DNA extraction displays clear and bright
distinct bands on the electrophoresis gel whereas low quality DNA presents a more
smeared appearance. DNA determination of gender shows as one or two distinct bands.
In mammals the male determines the sex of the offspring and has the
heterogametic XY genotype which presents as two distinct bands on a gel while
the female has the homogametic XX genotype and displays one distinct band on a
gel. In birds the genotypes are essentially opposite to mammals, the male has
the homogametic XX genotype showing one distinct band while comparatively the
female determines the sex of the offspring and has the heterogametic XY
genotype. To save confusion avian chromosomes have been classified in the ZW
sex determination system where males have the ZZ genotype and females have the
ZW genotype.
Sex determination in chickens is harder than mammals as
males and females are monomorphic, meaning they are not phenotypically
different in colour, body size or feather type etc. The following experiment
followed procedures outlined by Hogan, Loke & Sherman (2012) aiming to extract
a domestic chicken’s (Gallus Gallus) DNA
from three tissue types to determine the sex and to compare the quality and
quantity of DNA from the three samples. DNA was extracted using a commercial
DNA purification kit; DNeasy Blood & Tissue Kit produced by Qiagen (2012)
which is an expensive procedure however provides fast, easy and high yield
silica-based DNA purification utilizing Proteinase K which reduces mechanical
and contamination variable risks. The extracted DNA was amplified using PCR to
intensify the sex-specific locus CHD1W and CHD1Z, enabling us to determine the
gender of the bird using a set of universal avian sexing primers 2250F and
2718R developed by Fridolfsson and Ellegren (1999). Individual results were correlated
and compared to the class while molecular markers, negative, male and female
controls were used to determine whether the hypothesis was supported that the
more destructive and invasive techniques of the tissue and blood samples would
extract a higher DNA quality compared to the non-invasive technique of sampling
from a feather.
On completion of the procedure it was determined that Destructive
muscle sampling produced a higher yield of DNA compared to Invasive Blood
sampling with the lowest DNA yield for non-invasive feather sampling. Horvath,
Martinez-Cruz, Negro and Godoy (2005) have improved the extraction of DNA from
the feather tip by extracting blood from a blood clot located in the superior
umbilicus instead of the basal tip of the calamus which was used in the
author’s experiment. Their results indicate clot samples yielded a higher
amount of DNA than tip samples and less DNA degradation over time. This
procedure could increase the quantity and quality of DNA extracted in feather
samples in future experiments.
DNA Extraction from Blood, Feather and Muscle Samples
DNA extraction methods compromise of cell lysis which causes
a disruption in the cell membrane which allows proteins to be freed from the
cell. A protease may be added to remove the proteins and RNA removed with the
assistance of an RNAse. The DNA is then precipitated with an alcohol, then
amplified using PCR techniques and visualised using electrophoresis.
Following Hogan, Loke and Sherman (2012) in depth procedure
all materials and reagents were organised. A sterilized razorblade was used in
a sterile petri dish to reduce the muscle tissue down to form a smooth
consistency alternatively the superior end of the calamus of the feather was
sliced or a hole-punch sized piece cut out of the blood card. The samples were
then placed into a sterile microcentrifuge tube. All sharps were safely
discarded at this point. PBS (Phosphate Buffered Saline) and RNAse A was added
to the blood sample. Buffer ATL was added to the feather and muscle specimens
and all samples vortexed. Proteinase K was mixed through the specimens. The
blood sample was left to incubate for 30minutes at room temperature then all
specimens were incubated for 30 minutes at 56°C. During incubation the muscle
sample was vortexed every 10 minutes to aid in dispersion while 200µL
of Buffer AL was added to the blood sample. After incubation, RNAse was added
to the muscle sample, vortexed then incubated for a further 2min at room temperature
and vortexed again. The cells were lysed by this stage.
Buffer AL was added to the muscle and feather samples,
vortexed then 200 µL of ethanol was added to all samples which were vortexed again.
20µL of ethanol was added to the blood sample only allowing the solution to be properly
vortexed and become a homogenous solution allowing the DNA to precipitate and be
ready to be membrane bound.
The precipitated samples were pipetted into a labelled DNeasy Spin
Column/collection tube (Qiagen 2012) and centrifuged at 6000 x g (8000rpm) for
1 minute. The guanidine thiocyanate waste which remained in the collection tube
was discarded and a new collection tube attached. Buffer AW1 was added to the muscle
and feather samples. All samples were centrifuged for 1 minute at 6000 x g
(8000rpm) then Buffer AW2 was added and again centrifuged for 3 minutes at
maximum speed (13-14,000rpm) to dry the DNeasy membrane. The DNeasy mini spin
column was carefully removed so it did not come into contact with the ethanol
and guanidine thiocyanate waste and the collection tube replaced with a new
one. The sample was finally centrifuged for 1 minute at maximum speed to remove
any residual ethanol while the DNA was ready to be eluted from the membrane.
The collection tube was discarded and the DNeasy mini spin column
was placed into a labelled, clean, 1.5mL microcentrifuge tube. 100µL of Buffer
AE was pipetted directly onto the DNeasy membrane for the blood sample while
the feather and muscle samples had Buffer AE added in two 50µL steps the
samples were incubated at room temperature for 1 minute then centrifuged for a
further minute at 6000 x g (8000rpm) to elute. The elutant was kept aside. A
further 50 µL of Buffer AE was added to the membrane, incubated at room
temperature for 1 minute then centrifuged at 6000 x g(8000rpm). This elutant
was also kept aside. The two elutants were combined measuring 200 µL of DNA.
The column was discarded and DNA stored at -20°C until required.
Electrophoresis
Method
During
electrophoresis negatively charged DNA molecules migrated towards the positive
cathode causing smaller protein fragments to move quicker through the gel
matrix than larger molecules. The DNA was visualized as fragments in bands on
the gel which were stained with an intercalating agent, mutagen and suspected
carcinogen, Ethidium Bromide.
An agarose gel and TAE buffer was pre-prepared in the
microwave by boiling and allowing the gel to cool to 50 °C in a water bath. Using
gloves Ethidium Bromide was added to 150mL of gel to get a final concentration
of 0.5µL
mL-1. The casting tray was placed into the gel tank with black
casting gates at each end. The gel was poured into the tray and comb inserted
allowing 30 minutes for the gel to set at room temperature.
10µL of the DNA avian sample extracted
from the muscle earlier was mixed with the 6x loading dye in a clean microfuge
tube. Wearing gloves the black casting plates and comb was removed and TAE
buffer was added until the whole gel was covered by about 5mm.
The molecular weight markers ʎ HindIII and 2-log ladder were added into
the first and the last wells. The DNA samples were added into an empty well and
the position recorded. The electrophoresis unit was covered and connected to
the power unit and run at 120V for 60 minutes. The DNA proceeded to migrate
from the negative anode (black cable) to the positive cathode (red cable). Once
completed the gel tray was removed and transferred to a plastic container to
use the Gel Doc System so the Gel photos could be recorded and visualized (See
Figure 1).
PCR method
The Polymerase
Chain Reaction (PCR) procedure was used to amplify the DNA into a measureable
amount which could then be visualised using electrophoresis. PCR used a number
of reagents to cut specific sites of DNA which was then purified and used for
biological use. The PCR procedure consisted of cycles of heating and cooling
the DNA to allow helix unwinding and binding. Each complete cycle consisted of
the following: 1 cycle of 94°C for 5 minutes, 35 cycles of 94°C
for 30 sec, 55°C for 30 sec and 72°C for 30 seconds & 1 cycle of 72°C
for 5 minutes.
In order for PCR to be successfully carried out the DNA template
needed to be within a range of concentrations and be freed of inhibitors. This
was done by adding 10-100ng of DNA to a 50µL PCR product. If the band on
the gel was very faint or not visible the DNA solution was not diluted, if the
band was very bright the DNA was diluted by 1:5 with sterile MilliQ water.
The Mastermix, positive and negative controls were prepared as per
instruction in Hogan, Loke & Sherman (2012) and 40µL of the PCR mastermix and 10µL
of the DNA sample was mixed into a 0.2mL PCR tube. The prepared tubes were
placed into a thermo-cycler and a program which was optimised to amplify the
CHD1W and CHD1Z gene variants with the 2550F -2718R primer set.
Once the PCR product had been amplified the DNA was then run for 20
minutes at 300V on a 1% agarose gel in a 1 x SB electrophoresis buffer which
had been boiled and allowed to cool to 50°C. Wearing gloves 15µL
of 5mg mL-1 Ethidium Bromide stock solution was added to 150mL of SB
gel to achieve a final concentration of 5µg mL-1. The DNA
samples were prepared by mixing 10µL of PCR product with 4µL
of 6x loading dye and pipetted into the gel alongside 5µL of a 100bp molecular marker.
(See Figure 2)
The bands were again visualised using the Gel Doc System and PCR
product sizes were determined by comparing the position of the PCR band to the
molecular marker. (See Figure 2)
Figure 1:
(Right click on image to open in new tab) Class results for DNA extraction for various DNA samples. DNA was extracted
from blood, feather or muscle and visualised via electrophoresis.
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In Figure 1, DNA can easily be visualized from muscle wells (2, 8, 10,
12, 15 & 16) and from Table 1 and 2 muscle samples had ranging DNA
concentrations between 3.2-12.4ng/mL, and an average of 6ng/mL. Figure 1 shows DNA
is moderately visualized in blood wells (3, 5, 7, 11 & 14) and from table 1
and 2 blood samples range of DNA concentrations lay between 0-4.5ng/mL with an
average of 2.18ng/mL. Blood wells 3 and 14 had unknown concentrations as bands
were not visualized. From Figure 1, Feather wells (4, 6, 9 & 13) bands were
also moderately visualized while table 1 and 2 shows feather sample DNA
concentrations ranged from 0-3.2ng/mL with an average of 2.4ng/mL. Well 6
concentrations were unknown. Some samples within each tissue type yielded a
higher quality of DNA than others however on average muscle showed higher DNA
quality to blood and feather.
Table 1: (Right click image to open up in new tab) shows DNA samples
loaded in the wells, µL of sample loaded, referenced MWM of DNA in referenced
band and final concentration of DNA (ng/mL)
Well
|
Concentration
(ng/mL)
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Tissue
type
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Average
(ng/mL)
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16
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3.2
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Muscle
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6
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8
|
4.5
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15
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4.5
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2
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5.7
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12
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5.7
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10
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12.4
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6
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0
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Feather
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2.4
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4
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3.2
|
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9
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3.2
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13
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3.2
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||
3
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0
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Blood
|
2.18
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14
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0
|
||
5
|
3.2
|
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7
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3.2
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||
11
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4.5
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In Figure 2, Wells 2-9A, 11A, 12-14A, 18-19A, 2-5B, 9-11B DNA was
amplified and visualized successfully. Well 10A no DNA was extracted. Well
2B-8B show DNA samples, however controls were not consistent with others. Well
5B shows bottom band was more preferred than top band. Well 2B shows bands that
are not comparable to other blood samples as they are very faint. All samples
except 10B correlated with the actual sex of the individual, sample 10B was a
known male however bands were not representative of this.
Figure 2: (Right click image to open up in new tab)Class results for
various PCR product samples. DNA was amplified from DNA extraction and
visualized via electrophoresis to determine sex of bird. Results indicate an
error occurred in wells 1B-8B as controls are not as dark as what they were
expected to be indicating an error with PCR mastermix. Despite the error the
sexes were still able to be determined. PCR result matched expected result for
all samples except well 10B which was a known male.
Table 3: wells
corresponding to Figure 2, showing each sample number, tissue type, sample type
and well number reference from Figure 1.
Universal Primers 2550F and 2718R used in Fridolfsson and Ellegren
(1999) were replicated in the author’s procedure. Fridolfsson and Ellegren
(1999) developed the 2550F primer which binds to 5’-GTTACTGATTCGTCTACGAGA-3’
while the 2718R primer binds to 5’-ATTGAAATGATCCAGTGCTTG-3’ fragments of DNA
which were used to amplify sex specific loci; CHD1W & CHD1Z to determine
the gender of each sample taken. The advantages of employing universal sexing
molecular markers are the ability of the CHD1W and CHD1Z loci to be easily visualized
on a gel as they differ by 100-150 base pairs. According to Fridolfsson and
Ellegren (1999) the CHD1W fragments varied between 400-450 base pairs compared
to the CHD1Z fragments varying between 600-650 base pairs which were comparable
to replicated results. The samples were then compared to known male, female and
negative controls to view results and inconsistencies. Amplification of the
female chromosomes displays one CHD1W and one CHD1Z fragments on a gel compared
to the male chromosome of one CHD1Z fragment.
The authors experiment matches that of Fridolfsson and Ellegren (1999)
except that a 1% agarose gel was used to visualize the DNA fragments via
electrophoresis compared to Fridolfsson and Ellegren utilizing a 3% agarose
gel. They also used a phenol extraction according to Manniatis et al. (1982)
standard methods compared to our use of a commercial DNA purification kit.
(Qiagen 2012). Despite the differences our results were comparable to Fridolfsson
and Ellegren (1999).
The results show average sample DNA concentrations vary between tissue
types. Possible errors for non-reliable results include pipetting errors,
contamination, deviation from the method, a heterogeneous solution when
extracting the DNA from the sample and varying DNA quality from samples. The
results were also non representative between tissue types as the sample size
was small allowing no reliable comparisons to be made between genders within
specific tissue samples groups. Storage of DNA could also contribute to varying
DNA qualities as there were 6 weeks between the initial extractions of DNA and
recording the results from the PCR product. DNA was also stored at room
temperature during the practical classes contributing to slight gradual DNA
degradation even though ice was provided. This would not have affected the
visualised results as all samples were exposed to the same conditions.
Results indicate various samples did not compare to the majority. From
table 2, results indicate the average DNA concentration reflects muscle had the
highest quality of extracted DNA compared to feather, then blood however the
sample sizes were not equally distributed. The class contained 6 muscle
samples, 4 feather samples and 5 blood samples. As 1 feather sample and 2 blood
samples failed to extract any visible DNA (see figure 1) they bring the
averages down. By omitting the non-visible results (as all samples were able to
amplified by PCR so non visualized DNA could be due to lower than average DNA
quality) the average sample DNA concentrations reflect muscle still had the
highest quality of extracted DNA compared to blood then feather having the
lowest DNA quality which correlated to expected outcomes.
The three samples that failed to be visualized on the agarose gel
during the first round of electrophoresis following initial DNA extraction were
Blood well 3 sample B12.23, blood well 14 sample B12.21 and feather well 6
sample F12.20 (Figure 1). Figure 2 shows blood well 3 sample B12.23 was loaded
into well 11A where PCR was successfully able to amplify the minute amount of
DNA which resulted in a female bird with a more preferred W chromosome which
was represented by a darker bottom band (400-500bp) compared to the Z
chromosome top band. (600-700bp)
Feather well 6 sample F12.20 from figure 1 shows DNA was able to be
amplified to determine the sample was a male via PCR and visually represented
in Well 4A in Figure 2. The Z chromosome bands are very faint therefore further
PCR amplification would have been beneficial to increase the intensity of the
band.
Blood well 14 sample B12.21 from figure 1 shows PCR was also able to
successfully amplify the DNA sample but more amplification was required to
intensify the bands as Figure 2 shows two very faint bands representing the
female ZW genotype.
Other anomalies represented by the results include figure 2 displaying
the female feather sample F12.19 bottom W chromosome band (400-500bp) being
more preferred by the genotype than the Z chromosome band (600-700bp). This
sample is also slightly better visualized than most other feather samples. This
could be contributed to the amount of blood available in the tip or the
thickness of the stalk.
In muscle sample M12.27 in well 16 from figure 1 and well 5B in figure
2 shows the DNA quality and two chromosome bands which were very faint compared
to other muscle samples. The DNA extracted from the first electrophoresis
displays the lowest DNA concentration of the 6 samples indicating that the
amount of muscle may have been less or the muscle was not completely dissolved
into a homogenous solution. In comparison the amount of DNA extracted from
M12.27 was comparable to the amount of DNA extracted from the feather and blood
samples allowing the DNA to be amplified during PCR and allowing the genotype
to be determined. M12.27 banding patterns indicated in figure 2 show a female
with a preferred W chromosome than the fainter Z chromosome.
The male, female and negative controls in Well 6B-8B (Figure 2) are
not representative of other control samples. The preparation of the PCR
Mastermix was done according to the procedure outlined in Hogan, Loke &
Sherman (2012) and added to samples in Figure 2 represented in well 3B first
then well 4B, 2B and 5B then controls. Due to bubbles forming in the PCR
mastermix after addition to the first two samples, the adequate amount was not
able to be added to the remaining micro tubes resulting in fainter or
non-existent bands. The controls in Wells 6A-8A were used to compare samples
loaded in 2B-5B and 9B-11B.
Well 9 (Figure 1) and Well 10B (Figure 2) represents a male feather
sample F12.18. Table 1 indicates the most common amount of DNA was extracted
from the sample and successfully visualized in Figure 1. Figure 2 displays
multiple bands which are not representative of the known male genotype
indicating the sample was contaminated.
The above user errors could be avoided in future experiments by
adopting Taberlet et al’s (1996) procedure by introducing a multiple tube
approach, this would allow lower DNA yields to be rejected in line with Morin
et al. (2001) which although would be costly and require more reagents/kits it
would eliminate various user errors and produce more reliable results.
The duration of the experiment was held over 6 weeks therefore storage
of the DNA was considered. DNA can degrade overtime. Various methods of DNA
preservation discussed by Freeland (2005) indicate the importance of preserving
DNA to avoid DNA molecular arrangements being rearranged which can affect the
results when the DNA is amplified by PCR. Freezing at -20°C
was used to preserve the DNA samples in between each practical component. This
storage type is one of the most successful according to Colton and Clark
(2001). During each practical session the DNA was mostly stored at room
temperature which may have contributed to some DNA degradation however this was
unlikely to contribute to variations of DNA quality as all samples were exposed
to the same environments. During the practical elements ice esky’s were
provided to store the DNA samples however it was noted that all students kept
the DNA at room temperature when the DNA was not being used, this could be
avoided in future experiments by reminding the students of the importance of
preserving the DNA for extraction quality.
The quality of DNA extracted varied between tissue samples however all
sample types were able to be amplified utilizing PCR indicating non-invasive
techniques of using DNA from a feather could be used to extract DNA when alternative
methods are not suitable. Destructive muscle samples yielded the highest
quality and quantity of DNA compared to the other techniques however
destructive means of DNA extraction require the killing of the organism which
is not always suitable especially when dealing with endangered species.
Invasive blood sampling also produced a good yield and quality of DNA however
not as high as tissue sampling but could be used when tissue samples are not
available. Disadvantages of blood sampling include the requirement of capturing
the organism to extract a blood sample and samples are affected by storage
techniques as most samples are taken in the field. Non-invasive feather
samples, although yielding a lower DNA quality than the other samples the DNA is
easily obtainable in the field through capture and plucking of feathers of the
animal (Mundy et al. 1997) or obtaining specimens from the ground or nests.
(Beck, Double and Maurer 2010)
References
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