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DNA Barcode: species/varietal
         identification

Dr.N.Senthil
Professor (Biotechnology)
www.tnaugenomics.com
How the DNA Barcoding done
Molecular phylogeney




•   Molecular phylogeney has clarified many uncertainties in our view of
    species relationships and is particularly important in the study of
    evolutionary relationships between small and microscopic organisms (such
    as some insects, nematodes, protozoa and bacteria) which are vitaly
    important for ecosystems but where morphological features are difficult to
    identify and compare.
Why to barcode
• The total number of unique organisms described to the species
  level is around 1.5 million, but the total number of ‘species’ is likely
  to be in the region of 10 million.
• The overall ‘taxonomic deficit’ (the ratio of expected taxa to named
  taxa) is thus approximately sixfold.
• For vertebrates, the current described species total is likely to be
  relatively close to the ‘true’ total: we have described most of these
  relatively large organisms. The same is true of most groups whose
  members have body sizes greater than 10 mm.
• However, the vast majority of organisms on the Earth have body
  sizes less than 1 mm, and for these groups the taxonomic deficit is
  likely to be several fold worse than for land plants and vertebrates.
Species identification
• To provide a central catalog of organismal diversity
  which can be accessed by anyone who needs to quickly
  and accurately indentify an organism.
• Such a catalog would also allow us to differentiate new,
  previously undescribed species from those already
  observed and might represent a valuable tool in
• conservation efforts, the diagnosis of diseases, the
  monitoring of invasive species (those that colonize new
  environments to the detriment of native species), and
  many other fields.
DNA sequence -Barcode
• To gain an accurate picture of evolutionary
  relationships, it is usually neccessary to obtain
  the DNA sequence of many different genes from
  the organisms under study and compare them
  simultaneously.
• The technology required to isolate the part of the
  DNA of an organism that contains a gene of
  interest and determine its sequence (made up
  the the bases A, G, C and T) has recently become
  widely accessible, cheap and easy to master.
Isolation of specific gene
• A-priori, the sequence of two sequences near the ends
  of the gene (in practice this means that the gene
  should contain at least two short regions that are
  highly conserved between ALL species, while the rest
  of the sequence should be highly variable).
• Molecular biologists who have identified a gene called
  coxI , (cytochrome oxidase I) which seems to satisfy the
  requirements .
• CoxI (Cytochrome c oxidase subunit I )gene is found in
  the mitochondria of animals, plants and fungi
• Ribulose-bisphosphate carboxylase and Maturase K
  genes in plants (MatKi gene) from chloroplast origin
How to make reference sample and
        reference sequence ?
• The provision of specimens for the reference
  collection, and the correct linking of sequences to
  species in the reference collection.
• To this end, museums are providing access to their
  collections and their expertise in classical taxonomy,
  while significant funding is now dedicated to the
  isolation and sequencing of DNA from species that are
  not present in museum collections (as well as their
  taxonomic classification).
• Thus, barcoding has sparked a renaisence of interest in
  taxonomic studies.
DNA barcoding
• DNA barcoding is a technique for
  characterizing species of organisms using a
  short DNA sequence from a standard and
  agreed-upon position in the genome.
• DNA barcode sequences are very short
  relative to the entire genome and they can
  be obtained reasonably quickly and
  cheaply.
• The cytochrome c oxidase subunit 1
  mitochondrial region (COI) is emerging as
  the standard barcode region for higher
  animals.
• It is 648 nucleotide base pairs long in most
  groups, a very short sequence relative to 3
  billion base pairs in the human genome
Barcode’ metaphor
• All the products of one type
  on a supermarket shelf (like a
  2-litre bottle of Coca-Cola)
  share exactly the same 11-
  digit barcode, which is distinct
  from all other barcodes.
• DNA barcodes vary among
  individuals of the same
  species, but only to a very
  minor degree.
• If the DNA barcode region is
  effective, the minor variation
  within species will be much
  smaller than the differences
  among species.
Barcoding projects 4 components
•   Specimens :Natural history museums, herbaria, zoos, aquaria, frozen tissue
    collections, seed banks, type culture collections and other repositories of
    biological materials are treasure troves of identified specimens.

•   The Laboratory Analysis protocol to obtain DNA barcode sequences from these
    specimens available .

•   Barcode of Life Database (BOLD) was created and is maintained by University of
    Guelph in Ontario. It offers researchers a way to collect, manage, and analyze DNA
    barcode data.
•   The Data Analysis: Specimens are identified by finding the closest matching
    reference record in the database having Ribulose-bisphosphate carboxylase and
    Maturase K genes in plants
•   Animals :mitochondrial Cytochrome c oxidase subunit I gene

•   Fungal barcodes and accepts sequences from the Internal Transcribed Spacer
    Region
Selecting a core-barcode
   The standard animal CO1 DNA barcode fits
    the following criteria
    It is a haploid, uniparentally-inherited,
    single locus that shows high levels of
    discriminatory power
    It is a protein-coding region present in high-
    copy numbers per cell, and in animals
    it is not prone to drastic length variation,
    strong secondary structure,
   microinversions, or frequent
    mononucleotide repeats.
   well-developed primer sets
   CO1 sequences can be consistently
    orientated,
   Aligned with little supervision, and be
    translated to diagnose
   pseudogenes and identify sequencing errors.
Tools and Technology Required to
   Support DNA Barcoding in Plants
• Protocols and guidelines for DNA extraction and sequencing
  from herbarium specimens
• Continued improvement of PCR and sequencing protocols for
  regions rich in mononucleotide repeats
• Development of DNA barcoding primers and a system to
  record and predict which primers will work well in a given
  taxonomic group
• Development of robust multiplex PCR protocols
• Enhancement of mini-barcodes for degraded DNAs
DNA barcoding and its potential
• To establish a shared community resource of DNA sequences that
  can be used for organismal identification and taxonomic
  clarification.
• This approach was successfully pioneered in animals using a portion
  of the cytochrome oxidase 1(CO1) mitochondrial gene.
• In plants, establishing a standardized DNA barcoding system has
  been more challenging.
• The studies on cucumis sp for the application of DNA barcode
  shows the possibility of discrimination at species level not the
  varietal level using the matK gene barcode. The phylogenetic tree
  constructed by using matK gene sequences
• The barcode clearly differentiated the species C. sativus and C.
  melo which will help for the future application in cucumis taxonomy
  and phylogeny studies
Different markers in plant barcoding studies
DNA barcoding in plants
Genes used as Plant DNA barcode
Intraspecific gene flow on species discrimination success
DNA barcoding projects underway
Project and Lead Institute
• TreeBOL: Barcoding the world’s tree species :The New York
    Botanic Garden
• GrassBOL: Barcoding grasses and grass-like plants :Adelaide
    University and University of British Columbia
• Flora of the Kruger: National Park University of Johannesburg
• Flora of the Area de Conservacion Guanacaste :Costa Rica
    University of Pennsylvania
• Flora of Korea: Korea University
• Plant Barcoding China: DNA barcoding of 5000 Chinese plant
    species Kunming Institute of Botany
• All-genera: DNA barcoding of representatives of all angiosperm
    genera The New York Botanic Garden
• DNA barcoding of Centre for Tropical Forestry Plots
    :Smithsonian Institute
• DNA barcoding Chinese medicinal plants :Institute of Medicinal
    Plant Development Beijing
• DNA barcoding the flora of Wales :National Botanic Garden of
    Wales
• DNA barcoding British bryophytes :Royal Botanic Garden
    Edinburgh
BARCODE Applications
1) Geographically focused studies aiming to distinguishing among the
    diversity at a given site or region, where many of the samples are not
    necessarily closely related, and particularly where juvenile material and
    plant fragments require identifications; (
2) species in trade, where the challenge is often to distinguish between a set
    of target species, and often distantly related potential substitutes or to
    identify members of higher taxonomic groups (e.g. family, genus) rather
    than particular species; and
(3) where the identification problem relates to unfamiliarity with a given
    species such that the user may have no idea even what family a given
    species belongs to. In this situation, identification to a group of related
    species is useful as it can narrow down the total range of possible
    alternatives and also enable targeted use of morphological keys or expert
    consultation to obtain a final identification where required.
4) This ‘species group identification’, followed by subsequent ‘tie-breaker’
    analyses is particularly likely to be useful in species-rich systems where
    there is a shortage of available taxonomic expertise.
Future of DNA barcode


• Ecological forensics, identification of traded materials, undertaking
  identifications where there is a shortage of taxonomic expertise
  available, and assisting species discovery in some plant groups.
• Future technological advances will undoubtedly lead to
  improvements over current approaches
• Assembling large DNA sample sets representing the earth’s botanical
  diversity, supported by voucher specimens, and indexed via DNA
  sequences.
• This will provide the framework for current applications, and future
  developments, in the coordinated use of DNA sequence data to tell
  plant species apart.
BARCODE standard
Voucher specimens
Reference records
Public database
IDS – Identification System
Musquito barcode –disease control
Barcoding life.org



• The CBOL database (www.barcoding
  life.org) has 404,146 records representing
  40,110 species, a small proportion of the
  total biodiversity on earth, but a
  remarkable achievement for the first four
  years of its existence.
Bar coding of Cucumis genus
Indian sub-continent : centre of origin for cucumber (Cucumis

   sativus L. var. sativus; 2n = 14) centre of diversity for melon

   (Cucumis melo L.; 2n = 24)

Narrow genetic base - cultivated species were developed from

   closely related parents - limits crop improvement

Genetic diversity - morphological and molecular markers

   Recently, comparison of DNA sequences has been extensively

   used to identify phylogenetic relationship among different plant

   species.
matK (Megakaryocyte-associated tyrosine kinase)


•   The plastid gene trnK has a 2.5 kb class II intron including a 1.5 kb open reading frame called
    matK. formerly known as orfK

•   It is least conserved of the plastid genes and have high rate of nucleotide substitution compared
    to other genes

•   Evaluation rate of matK gene was approximately three fold faster than the rbcL gene in
    Saxifragaceae family

•   The matK gene sequence has been widely employed in inter and intragenous
    phylogenetic analysis in different plant species.
Morphological dendrogram generated by using UPGMA method
           based on Euclidean distance coefficient
                                                     @ 12.74
Genetic diversity analysis at molecular level
        using matK gene sequences

    Sequence analysis of matK region
    • Partial sequence was obtained using the
      reverse primer matK-8R.
    • Final alignment - 611 positions from each
      genotype.
    • 77 variable sites
    • 26 were informative for parsimony analysis
Parsimony informative sites for matK gene sequences
Phylogenetic analysis




Neighbor joining (NJ) tree                 Maximum likelihood (ML) tree
Cost of Reagents and Disposables
                         Fresh/Frozen   Museum

    Tissue Sampling         $0.41        $0.41

    DNA Extraction          $0.34        $2.00

    PCR Amplification       $0.24        $0.48

    PCR Product Check       $0.35        $0.70

    Cycle Sequencing        $1.04        $2.08

    Sequencing Cleanup      $0.32        $0.64

    Sequence                $0.40        $0.80

    Total:                  $3.10        $7.11
DNA from                             Create BARCODE
          identified voucher                       reference record



            Refine taxonomy                         ID unknowns
                of group




                               Create BARCODE                   DNA from unidentified
   DNA from                                                      immature specimen
                               reference records
identified adult
    voucher               Associate immatures
                              with names                              Repository of
                                                                       provisional
                                                                        vouchers
                                ID unknowns
Refine taxonomy                                                       Add names to
    of group                                                           vouchered
                                                                       immatures
Producing Barcode Data
 Barcode data anywhere, instantly


                        • Data in seconds to
                          minutes
                        • Pennies per sample
                        • Link to reference
                          database
                        • A taxonomic GPS
                        • Usable by non-
                          specialists

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Use of DNA barcoding and its role in the plant species/varietal Identification

  • 1. DNA Barcode: species/varietal identification Dr.N.Senthil Professor (Biotechnology) www.tnaugenomics.com
  • 2. How the DNA Barcoding done
  • 3.
  • 4. Molecular phylogeney • Molecular phylogeney has clarified many uncertainties in our view of species relationships and is particularly important in the study of evolutionary relationships between small and microscopic organisms (such as some insects, nematodes, protozoa and bacteria) which are vitaly important for ecosystems but where morphological features are difficult to identify and compare.
  • 5. Why to barcode • The total number of unique organisms described to the species level is around 1.5 million, but the total number of ‘species’ is likely to be in the region of 10 million. • The overall ‘taxonomic deficit’ (the ratio of expected taxa to named taxa) is thus approximately sixfold. • For vertebrates, the current described species total is likely to be relatively close to the ‘true’ total: we have described most of these relatively large organisms. The same is true of most groups whose members have body sizes greater than 10 mm. • However, the vast majority of organisms on the Earth have body sizes less than 1 mm, and for these groups the taxonomic deficit is likely to be several fold worse than for land plants and vertebrates.
  • 6. Species identification • To provide a central catalog of organismal diversity which can be accessed by anyone who needs to quickly and accurately indentify an organism. • Such a catalog would also allow us to differentiate new, previously undescribed species from those already observed and might represent a valuable tool in • conservation efforts, the diagnosis of diseases, the monitoring of invasive species (those that colonize new environments to the detriment of native species), and many other fields.
  • 7. DNA sequence -Barcode • To gain an accurate picture of evolutionary relationships, it is usually neccessary to obtain the DNA sequence of many different genes from the organisms under study and compare them simultaneously. • The technology required to isolate the part of the DNA of an organism that contains a gene of interest and determine its sequence (made up the the bases A, G, C and T) has recently become widely accessible, cheap and easy to master.
  • 8. Isolation of specific gene • A-priori, the sequence of two sequences near the ends of the gene (in practice this means that the gene should contain at least two short regions that are highly conserved between ALL species, while the rest of the sequence should be highly variable). • Molecular biologists who have identified a gene called coxI , (cytochrome oxidase I) which seems to satisfy the requirements . • CoxI (Cytochrome c oxidase subunit I )gene is found in the mitochondria of animals, plants and fungi • Ribulose-bisphosphate carboxylase and Maturase K genes in plants (MatKi gene) from chloroplast origin
  • 9. How to make reference sample and reference sequence ? • The provision of specimens for the reference collection, and the correct linking of sequences to species in the reference collection. • To this end, museums are providing access to their collections and their expertise in classical taxonomy, while significant funding is now dedicated to the isolation and sequencing of DNA from species that are not present in museum collections (as well as their taxonomic classification). • Thus, barcoding has sparked a renaisence of interest in taxonomic studies.
  • 10. DNA barcoding • DNA barcoding is a technique for characterizing species of organisms using a short DNA sequence from a standard and agreed-upon position in the genome. • DNA barcode sequences are very short relative to the entire genome and they can be obtained reasonably quickly and cheaply. • The cytochrome c oxidase subunit 1 mitochondrial region (COI) is emerging as the standard barcode region for higher animals. • It is 648 nucleotide base pairs long in most groups, a very short sequence relative to 3 billion base pairs in the human genome
  • 11. Barcode’ metaphor • All the products of one type on a supermarket shelf (like a 2-litre bottle of Coca-Cola) share exactly the same 11- digit barcode, which is distinct from all other barcodes. • DNA barcodes vary among individuals of the same species, but only to a very minor degree. • If the DNA barcode region is effective, the minor variation within species will be much smaller than the differences among species.
  • 12. Barcoding projects 4 components • Specimens :Natural history museums, herbaria, zoos, aquaria, frozen tissue collections, seed banks, type culture collections and other repositories of biological materials are treasure troves of identified specimens. • The Laboratory Analysis protocol to obtain DNA barcode sequences from these specimens available . • Barcode of Life Database (BOLD) was created and is maintained by University of Guelph in Ontario. It offers researchers a way to collect, manage, and analyze DNA barcode data. • The Data Analysis: Specimens are identified by finding the closest matching reference record in the database having Ribulose-bisphosphate carboxylase and Maturase K genes in plants • Animals :mitochondrial Cytochrome c oxidase subunit I gene • Fungal barcodes and accepts sequences from the Internal Transcribed Spacer Region
  • 13. Selecting a core-barcode  The standard animal CO1 DNA barcode fits the following criteria  It is a haploid, uniparentally-inherited,  single locus that shows high levels of discriminatory power  It is a protein-coding region present in high- copy numbers per cell, and in animals  it is not prone to drastic length variation, strong secondary structure,  microinversions, or frequent mononucleotide repeats.  well-developed primer sets  CO1 sequences can be consistently orientated,  Aligned with little supervision, and be translated to diagnose  pseudogenes and identify sequencing errors.
  • 14. Tools and Technology Required to Support DNA Barcoding in Plants • Protocols and guidelines for DNA extraction and sequencing from herbarium specimens • Continued improvement of PCR and sequencing protocols for regions rich in mononucleotide repeats • Development of DNA barcoding primers and a system to record and predict which primers will work well in a given taxonomic group • Development of robust multiplex PCR protocols • Enhancement of mini-barcodes for degraded DNAs
  • 15. DNA barcoding and its potential • To establish a shared community resource of DNA sequences that can be used for organismal identification and taxonomic clarification. • This approach was successfully pioneered in animals using a portion of the cytochrome oxidase 1(CO1) mitochondrial gene. • In plants, establishing a standardized DNA barcoding system has been more challenging. • The studies on cucumis sp for the application of DNA barcode shows the possibility of discrimination at species level not the varietal level using the matK gene barcode. The phylogenetic tree constructed by using matK gene sequences • The barcode clearly differentiated the species C. sativus and C. melo which will help for the future application in cucumis taxonomy and phylogeny studies
  • 16. Different markers in plant barcoding studies
  • 18. Genes used as Plant DNA barcode
  • 19. Intraspecific gene flow on species discrimination success
  • 20. DNA barcoding projects underway Project and Lead Institute • TreeBOL: Barcoding the world’s tree species :The New York Botanic Garden • GrassBOL: Barcoding grasses and grass-like plants :Adelaide University and University of British Columbia • Flora of the Kruger: National Park University of Johannesburg • Flora of the Area de Conservacion Guanacaste :Costa Rica University of Pennsylvania • Flora of Korea: Korea University • Plant Barcoding China: DNA barcoding of 5000 Chinese plant species Kunming Institute of Botany • All-genera: DNA barcoding of representatives of all angiosperm genera The New York Botanic Garden • DNA barcoding of Centre for Tropical Forestry Plots :Smithsonian Institute • DNA barcoding Chinese medicinal plants :Institute of Medicinal Plant Development Beijing • DNA barcoding the flora of Wales :National Botanic Garden of Wales • DNA barcoding British bryophytes :Royal Botanic Garden Edinburgh
  • 21. BARCODE Applications 1) Geographically focused studies aiming to distinguishing among the diversity at a given site or region, where many of the samples are not necessarily closely related, and particularly where juvenile material and plant fragments require identifications; ( 2) species in trade, where the challenge is often to distinguish between a set of target species, and often distantly related potential substitutes or to identify members of higher taxonomic groups (e.g. family, genus) rather than particular species; and (3) where the identification problem relates to unfamiliarity with a given species such that the user may have no idea even what family a given species belongs to. In this situation, identification to a group of related species is useful as it can narrow down the total range of possible alternatives and also enable targeted use of morphological keys or expert consultation to obtain a final identification where required. 4) This ‘species group identification’, followed by subsequent ‘tie-breaker’ analyses is particularly likely to be useful in species-rich systems where there is a shortage of available taxonomic expertise.
  • 22. Future of DNA barcode • Ecological forensics, identification of traded materials, undertaking identifications where there is a shortage of taxonomic expertise available, and assisting species discovery in some plant groups. • Future technological advances will undoubtedly lead to improvements over current approaches • Assembling large DNA sample sets representing the earth’s botanical diversity, supported by voucher specimens, and indexed via DNA sequences. • This will provide the framework for current applications, and future developments, in the coordinated use of DNA sequence data to tell plant species apart.
  • 29. Barcoding life.org • The CBOL database (www.barcoding life.org) has 404,146 records representing 40,110 species, a small proportion of the total biodiversity on earth, but a remarkable achievement for the first four years of its existence.
  • 30. Bar coding of Cucumis genus Indian sub-continent : centre of origin for cucumber (Cucumis sativus L. var. sativus; 2n = 14) centre of diversity for melon (Cucumis melo L.; 2n = 24) Narrow genetic base - cultivated species were developed from closely related parents - limits crop improvement Genetic diversity - morphological and molecular markers Recently, comparison of DNA sequences has been extensively used to identify phylogenetic relationship among different plant species.
  • 31. matK (Megakaryocyte-associated tyrosine kinase) • The plastid gene trnK has a 2.5 kb class II intron including a 1.5 kb open reading frame called matK. formerly known as orfK • It is least conserved of the plastid genes and have high rate of nucleotide substitution compared to other genes • Evaluation rate of matK gene was approximately three fold faster than the rbcL gene in Saxifragaceae family • The matK gene sequence has been widely employed in inter and intragenous phylogenetic analysis in different plant species.
  • 32. Morphological dendrogram generated by using UPGMA method based on Euclidean distance coefficient @ 12.74
  • 33.
  • 34.
  • 35. Genetic diversity analysis at molecular level using matK gene sequences Sequence analysis of matK region • Partial sequence was obtained using the reverse primer matK-8R. • Final alignment - 611 positions from each genotype. • 77 variable sites • 26 were informative for parsimony analysis
  • 36. Parsimony informative sites for matK gene sequences
  • 37. Phylogenetic analysis Neighbor joining (NJ) tree Maximum likelihood (ML) tree
  • 38. Cost of Reagents and Disposables Fresh/Frozen Museum Tissue Sampling $0.41 $0.41 DNA Extraction $0.34 $2.00 PCR Amplification $0.24 $0.48 PCR Product Check $0.35 $0.70 Cycle Sequencing $1.04 $2.08 Sequencing Cleanup $0.32 $0.64 Sequence $0.40 $0.80 Total: $3.10 $7.11
  • 39. DNA from Create BARCODE identified voucher reference record Refine taxonomy ID unknowns of group Create BARCODE DNA from unidentified DNA from immature specimen reference records identified adult voucher Associate immatures with names Repository of provisional vouchers ID unknowns Refine taxonomy Add names to of group vouchered immatures
  • 40. Producing Barcode Data Barcode data anywhere, instantly • Data in seconds to minutes • Pennies per sample • Link to reference database • A taxonomic GPS • Usable by non- specialists