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Kelly Ramig

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Cottonwood Tree Populus trichocarpa. Goal of Immediate Project ... Extracted nuclear DNA from frozen leaf samples ... This linkage map was constructed for Family 13 ... – PowerPoint PPT presentation

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Title: Kelly Ramig


1
Development of a Framework Map to Identify
Candidate Genes Involved in Carbon Allocation and
Partitioning in Populus
  • Kelly Ramig
  • Knox College, Illinois
  • Mentor Lee Gunter
  • Environmental Sciences Division

2
Long-Term Project Interest Enhancing
Sequestration of Atmospheric Carbon Dioxide
  • Fossil fuel use and deforestation account for
    emissions to the atmosphere of between 7.1-7.6
    GtC/yr
  • Oceans and terrestrial biomass accumulate only
    about 4 GtC/yr of excess carbon emissions
  • Due to imbalance, the atmosphere accumulates
    about 3.0-3.6 GtC/yr

From Equity Watch A Climate Newsletter from the
South
3
Long-Term Project Interest Enhancing
Sequestration of Atmospheric Carbon Dioxide
  • Carbon Sequestration The ability of plants to
    take CO2 from the atmosphere and store it in
    sinks such as leaves, stems, and roots
  • Carbon Allocation Determination of where the
    carbon is stored
  • Genetic improvement of poplar plantations could
    result in storage of up to 1.2 GtC/yr

From Environmental Protection Agency
4
Why Populus?
  • Widely accepted as genetic model for woody,
    perennial plants
  • Most species hybridize and produce fertile
    progeny
  • Closely related to Arabidopsis
  • Small genome size roughly 520 Mbp
  • Genome sequence, BAC library, and Linkage Maps
    for several species and pedigrees available

Cottonwood Tree Populus trichocarpa
5
Goal of Immediate Project
  • Analyze segregation patterns of genetic markers
    in a large pedigree to determine marker position
  • Consolidate marker position information for a
    framework map allowing for future
    characterization of loci involved in carbon
    sequestration and allocation

6
Project
  • Extracted nuclear DNA from frozen leaf samples
  • Amplified specific genetic marker loci through
    PCR
  • Fluorescently labeled PCR product denatured and
    genotyped
  • Data analyzed with genotyping software

7
Pedigree
  • Mother (52-225) is a hybrid cross between P.
    trichocarpa and P. deltoides
  • Father (D124) is a pure individual from the
    species P. deltoides

P. deltoides
P. trichocarpa
  • This pedigree contains gt1,000 progeny available
    for genetic studies

8
Genetic Markers
  • Genetic markers are anonymous DNA segments used
    to determine genetic variability
  • Microsatellites A heritable and highly
    polymorphic segment of DNA consisting of a short
    repeated sequence (1 to 10 bp)
  • Microsatellite loci chosen based on segregation
    and position on map of related pedigree (Family
    13)

Example of Microsatellite Allele Segregation
9
Summary of Results
  • Of the 64 primers tested
  • 82 amplified
  • 9.4 showed no segregation
  • 91.6 showed segregating alleles
  • Of the 51 segregating loci
  • 59.3 were fully informative
  • 37.0 maternally informative
  • 3.7 paternally informative

Non-segregating
No amplification
Segregating
Amplification
10
Summary of Results
Locus P571 Parental Cross CC ( ?) x AB (?)
Locus O-202 Parental Cross AB (?) x AN (?)
Expected Mendelian Segregation of Alleles
A 50 B 50 C 100
A 75 B 25 Null 50
Observed Segregation Results
A 51.6 B 48.4 C 100
A 53.6 B 78.6 Null 46.4
  • Of the 51 loci observed 25 alleles in 13 of
    the loci show significant segregation distortion
  • (based on the Chi-squared statistical test for
    significant difference)

11
Genetic Map Development
  • Segregation among genetic loci allows
    determination of chromosomal position
  • This linkage map was constructed for Family 13
  • Arrows indicate some of the loci mapped with new
    pedigree

12
Conclusions
  • High percentage of amplification displays marker
    fidelity
  • High percentage of segregation shows a high
    degree of consistency across pedigrees
  • Segregation distortion most likely due to small
    sample size of progeny tested
  • Initial work completed for an eventual dense
    genetic map of a large pedigree
  • Information collected from 63 out of the gt200
    markers needed for a dense genetic map
  • 44 of the gt1,000 progeny tested

13
Future Work
  • Continue mapping other microsatellite markers in
    order to make a dense genetic map
  • Compare the map from this pedigree to other maps
    in order to assess marker fidelity
  • Use markers for future characterization of genes
    involved in carbon sequestration and allocation

14
Acknowledgements
  • This research took place over the fall semester
    of 2003 at the Oak Ridge National Laboratory.
    Thank you to the Environmental Sciences Division,
    especially the Plant Genomics Group for creating,
    organizing, and funding this project. Sincere
    thanks especially to Lee Gunter, Gerald Tuskan,
    Steve Difazio, Ton Ming Yin, and Sara Jawdy for
    their technical expertise.
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