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The Environment Institute
                   Where ideas grow




   Professor Alan Cooper
   Environmental genomics
Environmental genomics:
Rapid biodiversity assessment of any sample




      Australian Centre for Ancient DNA,
          The University of Adelaide
Environmental genomics:
             Current Funding




ARC LINKAGE project (2009). $0.5M,
plus industry contributions (ca. 0.6M) =
$1.1M
Future Fellowship (2009). $1M
What is ACAD?
• Internationally leading centre for study of preserved
  genetic information
• Expertise with multiplex analysis (many genes) of
  biologically complex, trace-level samples, and 2nd
  Generation Sequencing
• Able to use existing museum and herbaria collections to
  generate reference database of taxonomically ID’d taxa
• AQIS approved facility
• Suitable for forensics (standard and environmental),
  sedimentary, and water analysis
Individual (still-air) working rooms      • 3 Laboratories – incl. high-
                                            tech ancient facility, museum
                                            grade specimens, modern lab

                                            • Trambarn - AQIS approved
                                            • Positive air-pressure
                                            • UV sterilisation
                                            • Controlled personnel flow

                                            • 16 researchers
-20’C                                       • International visitors
workrooms                                   • Evolution, archaeology,
                                            biodiversity/climate change,
             Air
            shower                          forensics - collaboration with
                                            AFP, DEH, NGS,
                                         Air flow




              UV
                             Entry
ancient DNA lab
= ultra-low DNA environment
Environmental Genomics
• Takes advantage of massive increase in sequencing power of 2nd and
  now 3rd Generation sequencing to perform vertical genetic bar-coding
• Capable of working with diverse taxonomic groups rapidly and
  simultaneously – using deep (multi-marker) characterisation of genetic
  diversity within any sample.
• Do not need to know what is present a priori, and can map species
  across a broad scale (eg landscape, soil, water, complex samples),
  and without need for prior taxonomic knowledge
• De novo assessment of biodiversity, eg mining, developing world
• Rapid, powerful, high resolution - using flexible, standard platform
• Remove constraints (esp. time) of traditional morphological
  approaches, ideal for mining, primary industries
• Needs active involvement of existing taxonomic and ecological
  expertise to identify accuracy, and potential uses
What is 2nd Generation Sequencing?

• It is already out of date.
• Parallel analysis of millions of different DNA sequences
  using chip-based arrays, or microwells
• Very cheap per base. 1st human genome = $Bn, currently
  <$50k
• Produces massive amounts of data, only few % of current
  products analysed
• 3rd Generation released next year. Active moves to locate
  machine at Adelaide for metagenomics. Promises of
  human genome in 3 minutes, for $5k.
• Key constraint in this revolution in biological science – who
  is going to analyse the data??
3rd Generation Sequencing - Oxford Nanopore Technologies




a-hemolysin nanopore (ribbon diagram) with covalently attached cyclodextrin (teal)
transiently binds a DNA base (red) traversing the pore. A, G, T, C and CM are
separated according to charge and mass. No need for dyes, CCD cameras etc
Current partners
• PIRSA: Paul Heithersay – sediment-based survey of biodiversity
  across South Australia, focusing on plant and animal taxa
• Australian Federal Police: Paul Kirkbride – forensic analysis of soils for
  geographic predictions, evidence analysis
• SA Water: Chris Saint – microbial diversity of water systems, including
  re-use, de-salination plants, and reservoirs. Unknown pathogens
• SA Pathology: Hamish Scott, Tuckweng Kok (James Paton) –
  microbial diversity within hospital/medical systems, unknown
  pathogens
• DEH: Hugh Cross, Andy Lowe – analysis of herbarium specimens,
  grasses
• José Facelli – ecological interpretation of EG data vs field sites
• Biomatters Ltd (Geneious): Shane Sturrock – design and
  implementation of software interface between raw genomics output,
  and end-users. Training postdocs and PhDs in bioinformatics.
• Daniel Huson (MEGAN) – leading metagenomics analytical software
Sample extraction
Ancient DNA methods developed to extract trace signals from
complex biological samples – eg sediments, old bones (mostly
microbes), faeces

Bulk processing (eg sediments), and selective hybridisation or
primer-based capture techniques to pull out useful sequences from
high background levels. Connect to High throughput sequencing

Water = bulk processing and filtering, perhaps with semi-permanent
sensors (IPAS)

R+D on DNA extraction and isolation procedures
Informative loci
The environmental genomics approach harnesses
to power of genomics technology, by focusing the
amplified loci to contain only taxonomically
informative genes.
Candidate loci, and suitable databases, already
exist although generally short and with limited
coverage.
Examples include COI/12S/cytb (vertebrates,
invertebrates), 16S (bacterial), rbcL/trnL, matK
(plants).
We will use extra domains within these loci, and
additional loci (eg nuclear introns, vWF, RAG-1,
others) as necessary. The system has large
capacity.
Future directions




• Genographic project
         • newly collected material (!), needs rates and demographic analysis
Metagenomic studies of ancient
samples confirm that most of
the DNA is exogenous/microbial
Voucher specimens
The environmental signals must be identified
through comparison with voucher specimens – eg
taxonomically identified material. The same genetic
loci must be sequenced to allow identification

Suitable material includes museums, herbaria,
microbial cultures and collections – but new
samples will need to be gathered and processed
throughout the project
Current constraints
Need locally sited 2nd or 3rd Generation machine
Desperate need for bioinformaticians (students and
trained maths/engineers/physicists
PhD and postdocs
Acknowledgements

Kyle Armstrong
Paul Brotherton
Wolfgang Haak
Jeremy Austin
The Environment Institute
                         Where ideas grow




   Next Seminar: 16 October

   Assoc. Prof. Bronwyn Gillanders
   Giant Australian cuttlefish: a globally unique species
   under threat?

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Environmental Genomics

  • 1. The Environment Institute Where ideas grow Professor Alan Cooper Environmental genomics
  • 2. Environmental genomics: Rapid biodiversity assessment of any sample Australian Centre for Ancient DNA, The University of Adelaide
  • 3. Environmental genomics: Current Funding ARC LINKAGE project (2009). $0.5M, plus industry contributions (ca. 0.6M) = $1.1M Future Fellowship (2009). $1M
  • 4. What is ACAD? • Internationally leading centre for study of preserved genetic information • Expertise with multiplex analysis (many genes) of biologically complex, trace-level samples, and 2nd Generation Sequencing • Able to use existing museum and herbaria collections to generate reference database of taxonomically ID’d taxa • AQIS approved facility • Suitable for forensics (standard and environmental), sedimentary, and water analysis
  • 5.
  • 6. Individual (still-air) working rooms • 3 Laboratories – incl. high- tech ancient facility, museum grade specimens, modern lab • Trambarn - AQIS approved • Positive air-pressure • UV sterilisation • Controlled personnel flow • 16 researchers -20’C • International visitors workrooms • Evolution, archaeology, biodiversity/climate change, Air shower forensics - collaboration with AFP, DEH, NGS, Air flow UV Entry
  • 7. ancient DNA lab = ultra-low DNA environment
  • 8. Environmental Genomics • Takes advantage of massive increase in sequencing power of 2nd and now 3rd Generation sequencing to perform vertical genetic bar-coding • Capable of working with diverse taxonomic groups rapidly and simultaneously – using deep (multi-marker) characterisation of genetic diversity within any sample. • Do not need to know what is present a priori, and can map species across a broad scale (eg landscape, soil, water, complex samples), and without need for prior taxonomic knowledge • De novo assessment of biodiversity, eg mining, developing world • Rapid, powerful, high resolution - using flexible, standard platform • Remove constraints (esp. time) of traditional morphological approaches, ideal for mining, primary industries • Needs active involvement of existing taxonomic and ecological expertise to identify accuracy, and potential uses
  • 9. What is 2nd Generation Sequencing? • It is already out of date. • Parallel analysis of millions of different DNA sequences using chip-based arrays, or microwells • Very cheap per base. 1st human genome = $Bn, currently <$50k • Produces massive amounts of data, only few % of current products analysed • 3rd Generation released next year. Active moves to locate machine at Adelaide for metagenomics. Promises of human genome in 3 minutes, for $5k. • Key constraint in this revolution in biological science – who is going to analyse the data??
  • 10. 3rd Generation Sequencing - Oxford Nanopore Technologies a-hemolysin nanopore (ribbon diagram) with covalently attached cyclodextrin (teal) transiently binds a DNA base (red) traversing the pore. A, G, T, C and CM are separated according to charge and mass. No need for dyes, CCD cameras etc
  • 11. Current partners • PIRSA: Paul Heithersay – sediment-based survey of biodiversity across South Australia, focusing on plant and animal taxa • Australian Federal Police: Paul Kirkbride – forensic analysis of soils for geographic predictions, evidence analysis • SA Water: Chris Saint – microbial diversity of water systems, including re-use, de-salination plants, and reservoirs. Unknown pathogens • SA Pathology: Hamish Scott, Tuckweng Kok (James Paton) – microbial diversity within hospital/medical systems, unknown pathogens • DEH: Hugh Cross, Andy Lowe – analysis of herbarium specimens, grasses • José Facelli – ecological interpretation of EG data vs field sites • Biomatters Ltd (Geneious): Shane Sturrock – design and implementation of software interface between raw genomics output, and end-users. Training postdocs and PhDs in bioinformatics. • Daniel Huson (MEGAN) – leading metagenomics analytical software
  • 12. Sample extraction Ancient DNA methods developed to extract trace signals from complex biological samples – eg sediments, old bones (mostly microbes), faeces Bulk processing (eg sediments), and selective hybridisation or primer-based capture techniques to pull out useful sequences from high background levels. Connect to High throughput sequencing Water = bulk processing and filtering, perhaps with semi-permanent sensors (IPAS) R+D on DNA extraction and isolation procedures
  • 13. Informative loci The environmental genomics approach harnesses to power of genomics technology, by focusing the amplified loci to contain only taxonomically informative genes. Candidate loci, and suitable databases, already exist although generally short and with limited coverage. Examples include COI/12S/cytb (vertebrates, invertebrates), 16S (bacterial), rbcL/trnL, matK (plants). We will use extra domains within these loci, and additional loci (eg nuclear introns, vWF, RAG-1, others) as necessary. The system has large capacity.
  • 14. Future directions • Genographic project • newly collected material (!), needs rates and demographic analysis
  • 15. Metagenomic studies of ancient samples confirm that most of the DNA is exogenous/microbial
  • 16. Voucher specimens The environmental signals must be identified through comparison with voucher specimens – eg taxonomically identified material. The same genetic loci must be sequenced to allow identification Suitable material includes museums, herbaria, microbial cultures and collections – but new samples will need to be gathered and processed throughout the project
  • 17. Current constraints Need locally sited 2nd or 3rd Generation machine Desperate need for bioinformaticians (students and trained maths/engineers/physicists PhD and postdocs
  • 19. The Environment Institute Where ideas grow Next Seminar: 16 October Assoc. Prof. Bronwyn Gillanders Giant Australian cuttlefish: a globally unique species under threat?