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For a greener future
Sachin S Rawat
School of Biotech, GGS IP University
A Look at the Plastid
A Plastid is a….
 Major organelle of plant and algal cells
 Site of manufacture and storage of important
chemical compounds
 Has circular, dsDNA copies
 Replicates autonomously of the cell
 Thought to have been originated from
endosymbiotic bacteria
 Plastid genes show maternal inheritance
Derived from proplastids in meristem
Have diverse functions
 Chloroplasts – green plastids – for
photosynthesis
 Chromoplasts – coloured plastids – for pigment
synthesis and storage
 Gerontoplasts – control dismantling of
photosynthetic apparatus during senescence
 Leucoplasts – colourless plastids – monoterpene
synthesis
 Leucoplasts include amyloplasts (starch),
elaioplasts (fats), proteinoplasts (proteins) and
tannosomes (tannins)
120-130 plastid genes
Are densely packed and fall into 2 categories:
 Photosynthesis-related genes
 Genetic system genes - genes for rRNAs, tRNAs,
ribosomal proteins and RNA polymerase subunits
A Fresher Look at the Plastid
Why plastid transformation?
 High protein expression levels
 Absence of epigenetic effects
 Uniparental inheritance is commercially favoured
 Easy transgene stacking in operons
 Increased biosafety – Since plastids are
maternally inherited, they aren’t transmitted by
pollen
Hurdles to ‘transplastomic’ plants
 Difficulty in delivering foreign DNA through double
membrane of the plastid
 The enormous copy number (polyploidy) of the
plastid genome
 The desired genetic modification must be in each
copy of plastid genome in each cell
 Failure to achieve homoplasmy results in rapid
somatic segregation and genetic instability
 Repeated rounds of selection and regeneration
are required
DNA delivery into plastids
 2 successful methods include biolistics and
polyethylene glycol-mediated transfer
 Biolistics is preferred as it is less time-consuming
and demanding
 Integration of foreign DNA into plastid genome
occurs via homologous recombination
 Homologous recombination operates in plastids
at a high efficiency
Biolistic chloroplast transformation and transgene integration into the
plastid genome via homologous recombination
Recent success
 Expression of Bt toxin gene from the tobacco plastid
genome
 High accumulation levels of Bt toxin protein (3-5 % of
TSP)
 Plants with high-level resistance to herbivorous insects
 Co-expression with upstream ORFs further increased
Bt toxin accumulation and even resulted in its
crystallization in chloroplast
 Production of somatotropin (7% TSP) in tobacco
plastids
Case Study I – Lactuca sativa
Protoplast isolation
 Lettuce seeds were sterilized and sown on MS
medium with 2% sucrose
 Shoot tips from leaves obtained were transferred
to MS medium with 3% sucrose
 The leaves were cut into pieces and incubated in
PG solution, followed by enzyme solution
consisting of 1% cellulase and .25% macerozyme
 Protoplast suspension was filtered through nylon
mesh
 Protoplasts were collected at surface after
centrifugation at 70g for 8min
Transformation and culture
 10µl transforming DNA and 0.6ml PEG solution
was added to protoplast suspension and incubated
at 25ºC for 10min
 Protoplasts were mixed with 1:1 solution of B5 and
2% agarose to a density of 3.6 X 104 protoplasts
per ml
 The suspension was plated onto Petri dishes and
cultured at 25ºC in the dark
 Selection was initiated on the 7th day by fresh
medium containing spectinomycin dihydrochloride
Analyses
 PCR – specific primers were used to assess the
presence of aadA gene in resistant cell lines
 Immunoblot analysis – using HRP-conjugated
secondary antibodies
 Southern and Northern blots were performed to
look for target genes and their transcripts
 After 2 weeks, non-transformants were yellow
while spectinomycin-resistant seedlings were
green and growing vigorously
 100% of spectinomycin-resistant lettuce cell lines
were true plastid transformants
 A limitation was the high frequency of polyploid
cell lines
Production of human
therapeutic proteins
Why lettuce is favoured over tobacco?
 Most of the plant is leaf tissue and this tissue
contains the greatest number of plastids per cell
 Unlike tobacco, lettuce has no toxic alkaloids that
need to be removed - low purification and
downstream processing costs
 Lettuce is a relevant human foodstuff that can be
consumed without cooking
Case Study II – Petunia hybrida
Plastid transformation
 Leaf pieces were placed on MS medium
supplemented with 1 mg/l 6-benzylaminopurine, 0.1
mg/l IAA, 30 g/l sucrose and 0.8% agar (MSB30)
 Leaves were bombarded with 1µm, vector-coated
gold particles from distance of 6cm
 Incubated in dim light for 48h at 25ºC
 Leaves were transferred to MSB30 medium with
200mg/l each of streptomycin sulfate and
spectinomycin dihydrochloride pentahydrate
 Resistant shoots first appeared after 8 weeks
Vector design
Analyses
 DNA blot – gene specific primers were used
 GUS assay – 5-Bromo-4-chloro-3-indolylbeta-D-
glucuronic acid was used to compare the protein
expression levels between the wild type and the
transformants by detecting fluorescence
 Selection on two antibiotics overcomes the
problem of spontaneous resistant mutants
associated with using spectinomycin alone
Comparing plastid
transformants with
non-transformants
Good model to study plastid biology
 N. tabacum is amphi-diploid
 A. thaliana doesn’t give rise to fertile
transplastomes
These limitations are overcome in Petunia as:
 P. hybrida is diploid
 Suitable for mutation screening to identify nuclear
loci affecting the maintenance and expression of
plastid transgenes
A Look at the Future
Metabolic pathways into plastids?
 Cost-effective production platform for
pharmaceuticals and nutraceuticals
 Production of trehalose in tobacco chloroplasts
 Tryptophan overproduction by feedback-
insensitive synthesis of α-subunit of anthranilate
synthase
 Simplifying technology, extending crop range
Can we engineer
photosynthesis?
 Efficiency of photosynthesis
 The most abundant protein in the world
 Its CO2:O2 specificity that matters
 Getting a better RubisCO for your plant
 Equally precise tools for nuclear genome required
Plastids for Synthetic Biology
 A compact, minimal genome
 High transgene expression and low cost ideal for
synthetic biology
 Designing totally new plastids
References
 Bock and Khan; Taming plastids for a green
future; Trends in Biotechnology
 Lelivelt et al.; Stable plastid transformation in
lettuce; Plant Molecular Biology
 Zuilen et al.; Stable transformation of Petunia
plastids; Transgenic Research
Thank you 

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Engineering the plastid

  • 1. For a greener future Sachin S Rawat School of Biotech, GGS IP University
  • 2. A Look at the Plastid
  • 3. A Plastid is a….  Major organelle of plant and algal cells  Site of manufacture and storage of important chemical compounds  Has circular, dsDNA copies  Replicates autonomously of the cell  Thought to have been originated from endosymbiotic bacteria  Plastid genes show maternal inheritance
  • 5. Have diverse functions  Chloroplasts – green plastids – for photosynthesis  Chromoplasts – coloured plastids – for pigment synthesis and storage  Gerontoplasts – control dismantling of photosynthetic apparatus during senescence  Leucoplasts – colourless plastids – monoterpene synthesis  Leucoplasts include amyloplasts (starch), elaioplasts (fats), proteinoplasts (proteins) and tannosomes (tannins)
  • 6. 120-130 plastid genes Are densely packed and fall into 2 categories:  Photosynthesis-related genes  Genetic system genes - genes for rRNAs, tRNAs, ribosomal proteins and RNA polymerase subunits
  • 7. A Fresher Look at the Plastid
  • 8. Why plastid transformation?  High protein expression levels  Absence of epigenetic effects  Uniparental inheritance is commercially favoured  Easy transgene stacking in operons  Increased biosafety – Since plastids are maternally inherited, they aren’t transmitted by pollen
  • 9. Hurdles to ‘transplastomic’ plants  Difficulty in delivering foreign DNA through double membrane of the plastid  The enormous copy number (polyploidy) of the plastid genome  The desired genetic modification must be in each copy of plastid genome in each cell  Failure to achieve homoplasmy results in rapid somatic segregation and genetic instability  Repeated rounds of selection and regeneration are required
  • 10. DNA delivery into plastids  2 successful methods include biolistics and polyethylene glycol-mediated transfer  Biolistics is preferred as it is less time-consuming and demanding  Integration of foreign DNA into plastid genome occurs via homologous recombination  Homologous recombination operates in plastids at a high efficiency
  • 11. Biolistic chloroplast transformation and transgene integration into the plastid genome via homologous recombination
  • 12. Recent success  Expression of Bt toxin gene from the tobacco plastid genome  High accumulation levels of Bt toxin protein (3-5 % of TSP)  Plants with high-level resistance to herbivorous insects  Co-expression with upstream ORFs further increased Bt toxin accumulation and even resulted in its crystallization in chloroplast  Production of somatotropin (7% TSP) in tobacco plastids
  • 13. Case Study I – Lactuca sativa
  • 14. Protoplast isolation  Lettuce seeds were sterilized and sown on MS medium with 2% sucrose  Shoot tips from leaves obtained were transferred to MS medium with 3% sucrose  The leaves were cut into pieces and incubated in PG solution, followed by enzyme solution consisting of 1% cellulase and .25% macerozyme  Protoplast suspension was filtered through nylon mesh  Protoplasts were collected at surface after centrifugation at 70g for 8min
  • 15. Transformation and culture  10µl transforming DNA and 0.6ml PEG solution was added to protoplast suspension and incubated at 25ºC for 10min  Protoplasts were mixed with 1:1 solution of B5 and 2% agarose to a density of 3.6 X 104 protoplasts per ml  The suspension was plated onto Petri dishes and cultured at 25ºC in the dark  Selection was initiated on the 7th day by fresh medium containing spectinomycin dihydrochloride
  • 16. Analyses  PCR – specific primers were used to assess the presence of aadA gene in resistant cell lines  Immunoblot analysis – using HRP-conjugated secondary antibodies  Southern and Northern blots were performed to look for target genes and their transcripts  After 2 weeks, non-transformants were yellow while spectinomycin-resistant seedlings were green and growing vigorously
  • 17.  100% of spectinomycin-resistant lettuce cell lines were true plastid transformants  A limitation was the high frequency of polyploid cell lines
  • 18. Production of human therapeutic proteins Why lettuce is favoured over tobacco?  Most of the plant is leaf tissue and this tissue contains the greatest number of plastids per cell  Unlike tobacco, lettuce has no toxic alkaloids that need to be removed - low purification and downstream processing costs  Lettuce is a relevant human foodstuff that can be consumed without cooking
  • 19. Case Study II – Petunia hybrida
  • 20. Plastid transformation  Leaf pieces were placed on MS medium supplemented with 1 mg/l 6-benzylaminopurine, 0.1 mg/l IAA, 30 g/l sucrose and 0.8% agar (MSB30)  Leaves were bombarded with 1µm, vector-coated gold particles from distance of 6cm  Incubated in dim light for 48h at 25ºC  Leaves were transferred to MSB30 medium with 200mg/l each of streptomycin sulfate and spectinomycin dihydrochloride pentahydrate  Resistant shoots first appeared after 8 weeks
  • 22. Analyses  DNA blot – gene specific primers were used  GUS assay – 5-Bromo-4-chloro-3-indolylbeta-D- glucuronic acid was used to compare the protein expression levels between the wild type and the transformants by detecting fluorescence  Selection on two antibiotics overcomes the problem of spontaneous resistant mutants associated with using spectinomycin alone
  • 24. Good model to study plastid biology  N. tabacum is amphi-diploid  A. thaliana doesn’t give rise to fertile transplastomes These limitations are overcome in Petunia as:  P. hybrida is diploid  Suitable for mutation screening to identify nuclear loci affecting the maintenance and expression of plastid transgenes
  • 25. A Look at the Future
  • 26. Metabolic pathways into plastids?  Cost-effective production platform for pharmaceuticals and nutraceuticals  Production of trehalose in tobacco chloroplasts  Tryptophan overproduction by feedback- insensitive synthesis of α-subunit of anthranilate synthase  Simplifying technology, extending crop range
  • 27. Can we engineer photosynthesis?  Efficiency of photosynthesis  The most abundant protein in the world  Its CO2:O2 specificity that matters  Getting a better RubisCO for your plant  Equally precise tools for nuclear genome required
  • 28. Plastids for Synthetic Biology  A compact, minimal genome  High transgene expression and low cost ideal for synthetic biology  Designing totally new plastids
  • 29. References  Bock and Khan; Taming plastids for a green future; Trends in Biotechnology  Lelivelt et al.; Stable plastid transformation in lettuce; Plant Molecular Biology  Zuilen et al.; Stable transformation of Petunia plastids; Transgenic Research