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Xspecies analysis of Aloe vera

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Title: Xspecies analysis of Aloe vera


1
Xspecies analysis of Aloe vera Oil Palm Zoe
Emmerson MRes in Advanced Genomic and Proteomic
Sciences 2009
2
Aims
  • Further proof of concept of the Xspecies method
    (Hammond et al., 2005).
  • Two species, Aloe vera and Oil Palm which are
    distantly related to Arabidopsis will be
    hybridised to the ATH1 GeneChip and the results
    assessed for conserved genes.

3
Introduction
  • Still many commercially and scientifically
    interesting species have little or no genome
    sequence available in the public domain.
  • Consequently, there are not many resources
    available for many important plant species which
    would aid, the understanding and conservation of
    the species.
  • However, there is an Abundance of resources
    available for the study of Arabidopsis.
  • Xspecies makes use of the already available
    technology for Arabidopsis and uses it to study
    other significant species.

4
The Three Species
  • Arabidopsis
  • Model organism
  • No economic value but many resources
  • Aloe vera
  • Native to sub-Saharan Africa, Arabian Peninsula
    and on some Indian Ocean islands
  • Adaptations such as succulent
  • Medicinal purposes for centuries
  • Huge economic value, markets worth millions of
    dollars.
  • Oil Palm
  • Originates in Africa
  • In-expensive food source and used in cosmetics
  • Large market Oil Palm produces the highest yield
    per hectare
  • Potential for use in biofuels

5
Phylogenetic Tree
The use of phylogenies is important for this
project because of the need to see the
evolutionary distance between the study species
A. vera, Oil Palm and the GeneChip species A.
thaliana.
Phylogeny of flowering plants (adapted from
Fawcett et al., 2009)
6
Introduction To Affymetrix Technology
  • Transcriptomics is the study of gene expression
    at the RNA level from the individual cell to
    whole tissues.
  • The transcriptome is dynamic and changes under
    the influence of the external environment and
    internal cues.
  • Affymetrix GeneChip highly reproducible due to
    mass production.
  • No need for technical replicates.
  • Cost effective and produces accurate data.
  • Each chip uses a probe set to represent each
    gene.
  • Instead of having a single oligonucleotide to
    represent each gene, the GeneChip uses between
    11 and 20 probe pairs depending on the species.
  • Each array contains multiple probe pairs in order
    to reduce the likelihood of random hybridisation
    and to increase the accuracy by using an average
    of the signal intensity across the probes.

7
The ATH1 GeneChip
  • The GeneChip that is to be used in this study is
    the Affymetrix Arabidopsis thaliana ATH1
  • ATH1 has 11 probe pairs, containing a perfect
    match (PM) and a mismatch (MM) probe.
  • The PM probes are precisely complementary to 11
    different 25 base pair sequences of the target
    gene.
  • The MM probe is the same an the PM with the
    exception of the 13th nucleotide that is altered
    so that the sequence is no longer an exact match
    for the target sequence of the gene. This is
    intended to be a built internal control for
    background hybridisation.
  • ATH1 GeneChip contains more than 22,500 probe
    sets which represent approximately 24,000 genes.
    The probe sets are scattered randomly across the
    surface of the chip to reduce the risk of losing
    entire probe sets in the case of uneven
    hybridisation, or damage to the surface of the
    chip.

8
Xspecies Method
  • The Xspecies method was developed by Hammond et
    al. (2005) as a response to the limited
    Affymetrix Genechip arrays available for a small
    number of plant and animal species.
  • Xspecies allows for increase sensitivity when
    used with heterologous species.
  • The specific Xspecies approach can greatly
    increase the number of potential genes that can
    be studied.
  • Holds great potential to enable the study of
    agriculturally or ecologically important plant
    species for which there is no GeneChip array
    available.

9
Materials Methods
10
Results
  • Shows that as the gDNA hybridisation intensity
    cut off increases the probe pairs and probe sets
    retained reduces.
  • This tells us the hybridisation effectiveness of
    the gDNA from the heterologous species to the
    ATH1GeneChip array.

11
Aloe Results
  • Volcano Plots
  • Aloe RNA hybridisation was filtered using the
    optimum .cdf 200 on a 1.5 fold change and with a
    P value of lt0.05 in order to pick out the
    statistically significantly altered genes and to
    reduce the gene set to a more manageable size.
  • This gave a result of 874 genes which were
    differentially regulated between leaf and root.
  • All further analysis was carried out on this
    smaller gene set.

12
Aloe Results
  • Principle Component Analysis (PCA)
  • 3 root replicates (blue) and 3 leaf replicates
    (pink) clustering at opposite ends of the graph.
  • This demonstrates that the 3 replicates of the 2
    tissue types have given similar results.
  • Simplified PCA, which shows a more definite
    separation of the two tissue types, root (blue)
    leaf (pink).

13
Aloe Oil Palm Results
Pink is up-regulated in Leaf, blue is
up-regulated in Root.
14
Results
  • Of the total of 13 genes involved in this pathway
    there are 6 found in Aloe and 12 in Oil Palm.
  • The 6 genes found in Aloe are common to all three
    species.

15
Results
  • There are 18 genes in this pathway which are
    found in Oil Palm.
  • Could be due to the large unfiltered gene set.

16
Results Venn Diagrams
Common to all 3 species 26 leaf genes involved
in photosynthesis.
6 root genes - metabolism processes
17
Gene Functions
  • The two most highly expressed genes in Aloe leaf
    have AGI codes
  • At4g26710 has the description of expressed
    protein and is a V-type H-ATPase, which is a
    response to salt stress gene. (Ratajczak, 1999).
  • At2g05070 is a light-harvesting chlorophyll a/b
    binding protein, which is integral to
    photosynthesis
  • The two most highly expressed genes in the Aloe
    root have AGI codes
  • At4g37370 is a cytochrome P450-like protein.
    Cytochrome P450 monooxygenases are a group of
    haem-containing proteins which catalyze various
    oxidative reactions (Naruskaka et al., 2004) and
    are involved in many metabolism processes.
  • At1g04820 is a Tubulin alpha-2/alpha-4 chain
    (TUA4) which is a general house keeping gene.
    Microtubules are essential in plants and play
    vital roles alpha tubulin is one of the building
    blocks of the microtubules in many plant
    developmental processes. Tubulins are found in
    all tissue types but are mainly found in root
    tissue (Dhonukshe, 2006).

18
C3'2009 2009 International Summer School on
Chips, Computers and Crops September 18th to
27th, 2009 Zhejiang University, Hangzhou, China
  • The summer school on Chips, computers and crops
    aims to teach best practice in the application of
    state-of-the-art computational techniques and
    genomic technologies to crop research.
  • The summer school covers interdisciplinary
    science, in a rapidly evolving field, bringing
    together ideas from the fields of mathematics,
    bioinformatics, genomics and post-genomic
    experiments on model organisms.

19
Some Findings From China
  • Several 6 base sequences occur in both
    Arabidopsis leaf and Aloe leaf, these have been
    identified to be involved in light
    responsiveness.
  • Of overlapping genes between Arabidopsis and Aloe
    some of the most significant are chloroplastic
    glutamine synthetase, and glutamate decarboxylase
    which is involved in glutamate metabolic
    activity. One paper suggests this is primarily
    expressed in the leaves and is important for
    assimilating ammonia released from
    photorespiration.
  • Of the genes more highly expressed in the roots
    of Aloe GO analysis found GO0000287 a magnesium
    ion binding gene.

20
Conclusions Further Work
This project has tested the Xspecies method, and
has shown that it is able to
  • Identify transcriptomic differences between leaf
    and root material.
  • Pick up genes highly up regulated in each
    material and allow further analysis e.g., GO
    ontologies and pathway searches.
  • Identifies genes common between target species.
  • Further Work
  • 2 more biological replicates for the Oil Palm
    leaf and root.
  • Include other species of plant to further
    validate the methods.
  • Hybridise both Aloe and Oil Palm to another
    monocot GeneChip such as the rice genome array.
  • Validation experiments would have to be carried
    out such as qPCR.

21
References
  • CHANG, S., PURYEAR, J. CAIRNEY, J. 1993. A
    Simple and Efficient Method for Isolating RNA
    from Pine Trees. Plant Molecular Biology
    Reporter, 11, 113-116.
  • DHONUKSHE, P., BARGMANN, B. O. R. GADELLA, T.
    W. J. 2006. Arabidopsis tubulin folding cofactor
    B interacts with alpha-tubulin in vivo. Plant and
    Cell Physiology, 47, 1406-1411.
  • FAWCETT, J. A., MAERE, S. VAN DE PEER, Y. 2009.
    Plants with double genomes might have had a
    better chance to survive the Cretaceous-Tertiary
    extinction event. Proceedings of the National
    Academy of Sciences of the United States of
    America, 106, 5737-5742.
  • HAMMOND, J. P., BROADLEY, M. R., CRAIGON, D. J.,
    HIGGINS, J., EMMERSON, Z. F., TOWNSEND, H. J.,
    WHITE, P. J. MAY, S. T. 2005. Using genomic
    DNA-based probe-selection to improve the
    sensitivity of high-density oligonucleotide
    arrays when applied to heterologous species.
    Plant Methods, 1, 10.
  • NARUSAKA, Y., NARUSAKA, M., SEKI, M., UMEZAWA,
    T., ISHIDA, J., NAKAJIMA, M., ENJU, A.
    SHINOZAKI, K. 2004. Crosstalk in the responses to
    abiotic and biotic stresses in Arabidopsis
    Analysis of gene expression in cytochrome P450
    gene superfamily by cDNA microarray. Plant
    Molecular Biology, 55, 327-342.
  • RATAJCZAK, R. 2000. Structure, function and
    regulation of the plant vacuolar H-translocating
    ATPase. Biochimica Et Biophysica
    Acta-Biomembranes, 1465, 17-36.

22
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