Post on 25-Apr-2020
Dianne Gleeson
The application of environmental DNA as a
biosecurity surveillance tool
What is eDNA?
• DNA that is left behind in the environment, sources
include water, soil, air, fecal etc
Methodology
eDNA Detection variables
Sensitivity depends upon:Volume of water, vs
Number of samples, ns
Number of aliquots, na
Proportion of template DNA per aliquot, ƒ
Developing quantitative framework
• Sensitivity depends upon:– θ, dispersion parameter
– λ, concentration of DNA
– ms , DNA molecules per water
sample
– mt, total molecules across all water
samples
– ma, no. molecules in an aliquot
– Xa, no. molecules amplified
– p, probability of successful
amplification of a target DNA
molecule
© Biosecurity SA
• Probability that no molecules will be
amplified in a single aliquot
P Xa = 0 | l > 0( ) =q
q + lvsns fp
æ
èç
ö
ø÷
q
• Probability that target DNA is
amplified in at least one aliquot
(detection)
Sensitivity = P Detection | l > 0( ) =1-q
q + lvsns fp
æ
èç
ö
ø÷
qna
Water
sample
Extracted
DNA
PCR
replicate
Amplification
Sampling Scheme
• 95% confidence in detection with varying no. samples, no. PCR replicates and concentration
• At a concentration of 10 molecules/litre, 95% detection probability will be achieved with 10 samples and 5 PCR replicates
na=1
na=2
na=3
na=4
na=10
.
.
.
.
Probability of Detection
Water samples required to achieve 95% confidence in detection
SPRING
0 5 10 15 20 25
0.0
0.4
0.8
Se
nsi
tivity
Carp
0 5 10 15 20 25
0.0
0.4
0.8
Se
nsi
tivity
Weatherloach
0 5 10 15 20 25
0.0
0.4
0.8
Number of samples
Se
nsi
tivity
Redfin
0 5 10 15 20 25
0.0
0.4
0.8
Se
nsi
tivity
Carp
0 5 10 15 20 25
0.0
0.4
0.8
Se
nsi
tivity
Weatherloach
0 5 10 15 20 25
0.0
0.4
0.8
Number of samples
Se
nsi
tivity
Redfin
AUTUMN
European carp control program, Tasmania
100x 600mL samples per lake. 6 qPCR replicates
Lake Sorell Lake Crescent
Lake volume (ML) 120,000 37,000
Carp population estimate 1140-1840 0
Positive eDNA samples 2/100 0/100
Positive qPCR replicates 2/600 0/600
Photo. J. YickPhoto. StudiaPhotos
Lake Sorell Lake Crescent
Lake volume (ML) 120,000 37,000
Carp population estimate 1140-1840 0
Num
ber
of
sam
ple
s
95% detection confidence assuming the current number of carp in the
lake is: Red line, at the lower population estimate (1140 carp) or blue line,
at the upper population estimate (1840 carp)
If 200 carp remain in Lake Sorell,
~7144 x 600mL eDNA samples are
required
Number of carp in Lake Sorell
1. Determined how soon can we detect eDNA after the introduction of the target species.
2. Developed methods for detecting spawning events
3. Investigated parameters for biomass detection of target species
4. Validation of molecular diagnostic assays of marine pests of high priority to Australia
5. Expanded assays for a range of non-fish species, including amphibians, reptiles, molluscs, crustaceans
6. Used high-throughput parallel sequencing to create species inventories from environmental samples
7. Investigating eDNA as tool for biocontrol agent detection
Subsequent studies/applications
http://www.smith-root.com/images/smith-root/edna/edna-process.png
Operationalising eDNA technology
Figure 1
The future of eDNA sampling & processing
Bohan et al. 2017 TREE
Global array of samples,
icloud network
reconstruction
Analysis across
highly replicated
networks
to detect change
Automated sampler
+ sequencing distributed
across global array
SAFA (CSIRO)
Sample Filtration &
Archival
In situ sampling device.
Automated collection of 24
samples, on site for later lab
analysis
MOBI (CSIRO)
Automated Realtime Algal ID
Microbial Oceanography Biosensing Instrument.
Fully automated, in situ instruments for DNA
analysis of water borne microbes.
eDNA for Border Biosecurity
• Commodity importation & real-time detection applications
• e.g Ornamental Fish Trade
Pest & Pathogen diagnostics
Cakechooser.com
Black tetra (Gymnocorymbus ternetzi)
Red belly piranha (Pygocentrus nattereri)
?
Research and Development Needs
• Improve the real-time detection technology
• Develop reference data-bases
• Establish standards and guidelines and QA/QC for application
Email: EcoDNA@Canberra.edu.au @Di_GleesonNZ