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Science and GMO-relevant technology

Science and GMO-relevant technology. Genes and genomes – last week Genomes and their inheritance and variation Genes and their structure Important methods: Gene cloning, PCR and microarrays Biotechnology - today Basic concepts of cloning/regeneration Transformation methods

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Science and GMO-relevant technology

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  1. Science and GMO-relevant technology • Genes and genomes – last week • Genomes and their inheritance and variation • Genes and their structure • Important methods: Gene cloning, PCR and microarrays • Biotechnology - today • Basic concepts of cloning/regeneration • Transformation methods • Transgene structure/expression

  2. Part I: Getting whole plants back from cultured cells • Organogenesis • Somatic embryogenesis

  3. Organogenesis – sequential differentiation of new plant organs (shoots, roots) First step is de-differentiation into callus after treatment with the plant hormone auxin Leaf-discs

  4. Shoots usually are produced first, then roots in organogenesis

  5. Somatic embryogenesis – shoot-root axis differentiated as a unit Immature cotyledon Somatic embryos Repetitive embryogenesis = cloning

  6. Somatic embryogenesis Embryo growth Dry-down for storage - propagation Physiological maturity

  7. Somatic embryogenesis Germination and plant recovery

  8. Part II: Getting DNA into plant cells Main methods • Agrobacterium tumefaciens • Biolistics [gene gun]

  9. Agrobacterium is a natural plant genetic engineer

  10. T-DNA Ti plasmid The Ti-plasmid is required for crown gall disease T-DNA = Transferred DNA Ti = Tumor inducing

  11. Opine Catabolism Cytokinin Synthesis Auxin Synthesis Right Border T-DNA Left Border 200000 bp Virulence region independent of T-DNA Opine Metabolism The Ti Plasmid Hormones cause gall growth, opines are special nitrogen sources

  12. Left Border Right Border Nick by VirD2 Nick by VirD2 New strand synthesis Strand displacement Vir E Vir E Vir E Vir E Vir E Vir E Vir E Vir E Vir E Vir E Vir E Vir E Vir E Vir E Vir E Vir E Vir E Vir E Vir E Vir E Vir E Vir E Vir E Vir E Agrobacterium transfer is complex Borders define start and end of T-DNA Preparation of T-strand Export out of the cell

  13. Disarming the T-DNA Border Border Auxin Synthesis Cytokinin Synthesis Opine Synthesis Cut and replace Antibiotic Resistance Gene of Interest Reporter Gene

  14. Promoter Terminator Coding sequence A chimeric gene • Polyadenylation site • Provides stability to mRNA • Level of expression • Constitutive • Tissue-specific • Mix and match parts

  15. Example of a map of plasmid used in plant transformation GUS gene encodes glucuronidase (cleaves pigment to make blue color): GUS reportergene enables easy visualization of successful transformation, and where and when genes are expressed

  16. T-DNA Ti Plasmid Gene of interest Agrobacterium engineering Engineered plant cell Agrobacterium tumefaciens

  17. Cocultivation of Agrobacterium with wounded plant tissues

  18. Agrobacterium in contact with wounded plant tissues during cocultivation

  19. The gene gun Plastic bullet DNA on gold particles Firing pin .22 caliber charge Stopping plate

  20. Gene gun bombardment of plant tissues in Petri dish

  21. DNA coated metal particles after “gene-gun” insertion into tissues

  22. Transgenic cassava via biolistics GUS reporter gene gives blue color

  23. Part III: Selection of transgenic cells

  24. Only a few cells get engineered Challenge: Recover plants from that one cell so new plant is not chimeric (i.e., not genetically variable within the organism)

  25. Hormones in plant tissue culture stimulate division from plant cells

  26. Antibiotics in plant tissue culture limit growth to engineered cells Other kinds of genes can also be used to favor transgenic cells (e.g., sugar uptake, herbicide resistance)

  27. Antibiotic selection of transgenic tissues in poplar

  28. Summary of steps in Agrobacterium transformation

  29. Analysis of transgenic plants Number of gene copies can vary Junction fragment analysis reveals number of gene insertion sites Restriction enzyme sites shown with arrows flanking DNA inserted gene flanking DNA

  30. Transgene structure and orientation can vary Single, simple copies much preferred for stability

  31. Transgene expression level varies widely between insertions (“events”) Partly due to failure to control where gene inserts in genome

  32. Interpreting significance of GE’s unintended effects on genome • Lots of unintended genetic change in breeding • Lots of genetic variation in gene content and organization • No urgency to regulate traditional breeding

  33. Varieties derived from induced mutations Over 2000 crop varieties derived from mutagenesis have been commercialized. Calrose 76 semi-dwarf rice High oleic sunflower Rio Red grapefruit

  34. Comparing GE to other breeding methods Expert view on chance of unintended consequences for food quality National Research Council (2004) http://books.nap.edu/execsumm_pdf/10977.pdf

  35. Extensive natural genetic diversity in gene structure/content (maize)Natural deletions of genes/chromosome sections

  36. Summary of some GE biological issues to consider • Events = unique gene insertion • They vary widely in level/pattern of expression due to chromosomal context / modification during insertion • The unit of regulatory consideration at present • Mutagenic changes at insertion site highly variable (deletions, duplications) • Can be “read-through” (Agro DNA beyond T-DNA transferred) • Stability of gene expression and gene silencing • A large number of insertions are not expressed • Some lose/change expression over time • Must select and test events carefully – single copy preferred

  37. LAG LSAG LSAG LAG Intron Summary of some GE biological issues to consider • Somaclonal variation = unintended mutagenesis due to tissue culture & regeneration system • Can be substantial, varies widely depending on culture system • Must weed out via crossing, intense selection of events • Increasing use of RNAi (RNA interference), as a general means of gene suppression in research and commerce • A way to knock out specific genes, inhibit viruses • Genes with inverted repeat DNA create double-stranded RNA, which induces sequence-specific RNA degradation or inhibition of translation – very active area of basic and applied research

  38. Discussion questions • What aspects of gene transfer are most unclear? • What are most important to understand for interpreting biotechnologies? • Should individual gene transfer events be the focus of safety evaluations? • Or should the type of gene in a specific crop be regulated instead? • Should GE crops that modify the expression of native kinds of genes (ie, not introduce novel kinds of genes) be regulated at all?

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