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01/01/2014 SAMI 1
PLANT
BREEDING
SELECTION
HYBRIDIZATION
INTRODUCTION
MUTATION
TISSUE
CULTURE
GENETIC
ENGINEERING
transgenics
UNIVERSITY OF AGRICULTURAL AND HORTICULTURAL SCIENCES, SHIMOGA.
COLLEGE OF HORTICULTURE, MUDIGERE.
 Introduction
 Transformation methods
 Practical application
 Herbicidal, Pest, Disease,
Drought – Tolerance, and
Quality
 Indian research
 Conclusion
01/01/2014 SAMI 3
Introduction
01/01/2014 SAMI 4
Biotechnology is one of the tools , but a
potentially important one, in the struggle to
reduce poverty, improve food security, reduce
malnutrition and improve livelihood of the rural
and the urban poor.
- Persley, 1999
 Modification of an organism’s DNA in order
to achieve a desired trait.
01/01/2014
SAMI
5
What are genetically modified organisms (GMO) ?
+ =
Arctic fish DNA Tomato
A tomato resistant to
frost
What is transgenic?
http://en.wikipedia.org/wiki/Fish_tomato
01/01/2014 SAMI 6
Brief history of transgenics
ISAAA, 2011
1985
1st
transgenic
plants
produced.
1994
Flavr-Savr
tomato is
released
1996
Herbicide-
and insect-
resistant
crops
approved
for
cultivation
2000
Golden rice
with
ß-carotene
developed
2011
160 million
ha. of GM
crops
planted.
GM crops
considered
substantially
equivalent to
hybrid
varieties
1992
01/01/2014 SAMI 7
How transgenic breeding
differs from conventional
breeding?
Conventional Breeding Transgenesis
Current cultivar Wild relative
GOI
Unwanted
genes
Back cross
F1 generation
F2 generation
Many backcrosses
New Cultivar
Unwanted
Genes
GOI
Current
Cultivar
Transfer in to
plasmid
agrobacterium
GOI
Genes
required
for transfer
& marker
genes
New Cultivar
Unrelated organism
Genes
required
for transfer
& marker
genes
GOI
01/01/2014 SAMI 8
TOMATO
• Most common vegetable
• Indian meals incomplete without tomato.
• Botanical name Solanum lycopersicum L.
• Chromosome number 2n = 24
• Well distributed throughout the world
• One among the top five vegetables
01/01/2014 SAMI 9
Area Production Productivity(t/ha)
INDIA 8.65 lakh ha. 16.82 lakh tons 19.5
KARNATAKA 51.2 thousand
ha.
1756.7 thousand
tons
19.5
Anon 2012
Source
– NBPGR, NCBI etc.,
Vector Construction
– Plasmid, cosmid, bacteriphage, virus etc.,
Transformations
– Microinjection, Gene gun, Electrophoretion, Agrobacterium, etc.,
Selection of transgenic plant (Antibiotic containing media)
Elimination of marker and backbone (through DEX media)
Confirmation (through PCR)
Expression
– Southern blotting, RT PCR, ELISA
01/01/2014 SAMI 10
01/01/2014 SAMI 11
Transformation Methods
Microinjection
Biolistics - gene gun/
particle bombardment
Electroporation
Silicon carbide fibers
PEG
DEAE-dextran
Calcium
phosphate
A. tumefaciens
A. rhizogenes
Virus-mediated
Pollen
transformation
Meristem
transformation
Singh B. D., 2009
01/01/2014 SAMI 12
Methods of plant transformation
PHYSICAL CHEMICAL BIOLOGICAL IN PLANTA
Agrobacterium mediated transformation
• Most extensively used method
• Natural ability of Agrobacterium to transfer plants
• First report: McCormick et al.(1986)
• Cotyledons/leaves are used for transformation
• A. tumefaciens and A. rhizogenes
01/01/2014 SAMI 13
Tomato transformation mediated by
Agrobacterium
01/01/2014 SAMI 14
01/01/2014 SAMI 15
Simple and efficient Agrobacterium mediated
procedure for transformation of Tomato
01/01/2014 SAMI 16
Bacterial strain used : A. tumefaciens strain AGL 1
Growth conditions-
Growth room temperature : 28 10C
Culturing of Agrobacterium : Rotary shaker (280C) for 72hrs at 200 rpm
Explants : Cotyledons from 10 day old plants
Size of explant : 0.7 cm x 1.0 cm
Varieties studied : Pusa Ruby, Arka Vikas and Sioux
Sharma et al., 2009, New Delhi
Figure 1 : Vectors used for transformation of Tomato using A. tumefaciens
strain AGL 1
(Sharma et al., 2009)
01/01/2014 SAMI 17
Plate 1: Different stages of Solanum lycopersicum var. Pusa Ruby
transformation
01/01/2014 SAMI 18
(Sharma et al., 2009)
Table 1: Effect of bacterial concentration and co-cultivation
period on transformation of Pusa Ruby
(Sharma et al., 2009)
01/01/2014 SAMI 19
Bacterial
concentration
No. of
explants
Averaga percent transformation
efficeincy + SE
72 h
cocultivation
96 h
cocultivation
0.5 X 108 70 20.7 + 1.01 22.1 + 1.01
1.0 X 108 70 41.4 + 2.02 24.3 + 2.02
2.0 X 108 70 38.6 + 2.02 19.3 + 3.03
5.0 X 108 70 36.4 + 1.01 17.9 + 1.01
10 X 108 70 12.9 + 2.02 -
Table 2: Transformation efficiency of different Tomato varieties
using optimized protocol
(Sharma et al., 2009)
01/01/2014 SAMI 20
Vector used Tomato
variety
Average No. of
explants co-
cultivated
Average transformation
efficiency (% + SE)
pCTBE2L Pusa Ruby 174 40.5 + 0.80
pRINASE2L Pusa Ruby 163 41.1 + 0.89
pCTBE2L Sioux 150 41.0 + 1.00
pCTBE2L Arka Vikas 150 22.0 + 1.50
Biolistic gun
• Most successfully applied
• Also known as ‘Particle bumbardment’
• Principle: High velocity discharge of DNA
‘bullets’ coated with gold or nickel particles
• Non specificity of species
• Gene integration is random
• Low rate of stable transformation (10-5)
01/01/2014 SAMI 21
Plate 2 : Gene gun
01/01/2014 SAMI 22
01/01/2014 SAMI 23
01/01/2014 SAMI 24
Tomato transformation using biolistic gun
• Intoduced gene : β glucuronidase (gusA)
• Genotype : IPA-3
• Explants : Shoot tips, hypocotyls and
cotyledon
• Particle gun used : Bio-Rad Gun
• TC media : MS + BAP (2.0 mg/l) + Kinetin
(1.0 mg/l)
01/01/2014 SAMI 25
Ruma et al., 2009, Ludhiana
Source df
Mean sum of squares
Target
distance
DNA
quantity
Pre-
bumbardment
culture
Post-
bumbardment
culture
Explant 2 210.71* 9.66 45.29* 8.24*
Parameters 3 1457.75* 1508.98* 772.85* 548.94*
Explant x
Parameters
6 37.12* 52.72* 1207.10* 3.21
Error 24 7.04 14.78 12.25 26.42
Table 3 : ANOVA for GUS expression as affected by different
parameters of particle gun
(Ruma et al., 2009)
Figure 2: Effect of target
distance on
transformation
01/01/2014 SAMI 26
Source df
Mean sum of squares
Target
distance
DNA
quantity
Pre-
bumbardment
culture
Post-
bumbardment
culture
Explant 2 210.71* 9.66 45.29* 8.24*
Parameters 3 1457.75* 1508.98* 772.85* 548.94*
Explant x
Parameters
6 37.12* 52.72* 1207.10* 3.21
Error 24 7.04 14.78 12.25 26.42
Table 4: ANOVA for GUS expression as affected by different parameters of
particle gun
(Ruma et al., 2009)
Figure 3: Effect of DNA quantity
on transformation
01/01/2014 27SAMI
Source df
Mean sum of squares
Target
distance
DNA
quantity
Pre-
bumbardment
culture
Post-
bumbardment
culture
Explant 2 210.71* 9.66 45.29* 8.24*
Parameters 3 1457.75* 1508.98* 772.85* 548.94*
Explant x
Parameters
6 37.12* 52.72* 1207.10* 3.21
Error 24 7.04 14.78 12.25 26.42
Table 5: ANOVA for GUS expression as affected by different parameters
of particle gun
(Ruma et al., 2009)
Figure 4: Effect of pre-bumbardment
culture on transformation
01/01/2014 SAMI 28
Source df
Mean sum of squares
Target
distance
DNA
quantity
Pre-
bumbardment
culture
Post-
bumbardment
culture
Explant 2 210.71* 9.66 45.29* 8.24*
Parameters 3 1457.75* 1508.98* 772.85* 548.94*
Explant x
Parameters
6 37.12* 52.72* 1207.10* 3.21
Error 24 7.04 14.78 12.25 26.42
Table 6: ANOVA for GUS expression as affected by different
parameters of particle gun
(Ruma et al., 2009)
Figure 5: Effect of post bumbardment
culture on transformation
01/01/2014 SAMI 29
Plate 2: Different explants showing GUS expresion
a. Cotyledons, b. Shoot tips, c. Hypocotyls, d. Leaf, e. Callus, f. Root like
structures
01/01/2014 SAMI 30
Pollen mediated transformation of
Tomato
01/01/2014 SAMI 31
01/01/2014 SAMI 32
Does not require tissue culture and plant
regeneration
Produces genetically uniform progeny
Not expensive
Genotype independent – monocots/dicots
Utilizes normal fertilization process
Benefits of pollen transformation
01/01/2014 SAMI 33
Bacterial strain used: A. tumefaciens strain
LBA4404
Growth conditions:
Growth room temperature : 28 ± 10C
Culturing medium : Yeast Extract Mannitol Agar
+ Streptomycin (100 µg/ml) +
Rifampicin (25 µg/ml) +
Kanamycin (50 µg/ml)
In vitro manipulation of pollen for
transformation in Tomato
Satish, 2009, Dharwad
(Satish, 2009)
01/01/2014 SAMI 34
Plate 3: Vector used for transformation
of pollen of Tomato
01/01/2014 SAMI 35
Table 7: In vitro pollen germination medium for Tomato (Pusa Ruby)
(Satish, 2009)
Medium Germination (%) Tube length (m)
PGM-1 32.00c 190c
PGM-2 46.80b 213b
PGM-3 92.96a 281a
CD @1% 1.62 1.00
Media constitution:
PGM-1: Sucrose (18%) + Agarose (1%) + Boric acid (0.015%)
PGM-2: Sucrose (16%) + Boric acid (0.6mM) + CaNO3 (0.8mM) +
MgSO4 (0.5mM)
PGM-3: Sucrose (10%) + Boric acid (100mg/l) +GA (125µM)
01/01/2014 SAMI 36
Herbicidal tolerance
Pest tolerance
Disease tolerance
Abiotic stress tolerance
Quality improvement
01/01/2014 SAMI 37
Engineering herbicidal resistance in plants by
expression of detoxifying enzyme
01/01/2014 SAMI 38
Block et al., 2007, England
Experimental details:
Bacterial strain used : A. tumefaciens strain C58C1 Rif
Variety used : Petit Havana
Explant : Leaf disc
Media (5.7 pH) : ½ MS + Sucrose (1%) + Agar
(0.8%)
Gene : bar gene
Mechanism : PAT (Phosphinothricin
acetyltransferace)
detoxification
Figure 6: Ammonia determination (% basal NH4
+ content) after
spraying Basta® (20 l/ha)
(Block et al., 2007)
01/01/2014 SAMI 39
Class of
herbicide
Compound/
Herbicide
Transgene/
Mechanism
Company
Phosphonic
acid
Phoshanothricin
(Basta®
, Liberty®
)
bar gene/ PAT
detoxification
Syngenta
Sulphonylurea
Chlorosulphuron
(Glean®
)
Mutant plant/
acetolactate
synthase
Dupont-
Poineer-Hi-
Bred
Nitriles
Bromoxynil
(Buctril®
)
Nitrilase
detoxification
Calgene/
Bayer crop
science
(Slater, 2010)
01/01/2014 SAMI 40
Genetic manipulation for pest tolerance
01/01/2014 SAMI 41
table 9: Different versions of the Cry genes effective
against different orders of insects
Cry gene designation
Toxic to these insect
orders
CryIA(a), CryIA(b), CryIA(c) Lepidoptera
Cry1B, Cry1C, Cry1D Lepidoptera
CryII Lepidoptera, Diptera
CryIII Coleoptera
CryIV Diptera
CryV Lepidoptera, Coleoptera
01/01/2014 SAMI 42
Byrne et al., 2002
Experimental details:
Bacterial strain used : A. tumefaciens strain LBA 4404
Variety used : Pusa Ruby
Explant : Cotyledonary leaves from 10-day old
seedlings
Media (5.7 pH) : ½ MS + Sucrose (1%) + Agar (0.8%)
Gene : cry1Ac gene
01/01/2014 SAMI 43
Transgenic tomato plants resistant to fruit borer
(Helicoverpa armigera Hubner)
Mandaokar et al., 2000, New Delhi
01/01/2014 SAMI 44
Mandaokar et al., 2000, New Delhi
Table 10: Expression of Cry 1 Ac protein in transformed Pusa
Ruby
Plant no. Cry1Ac content(% of total
soluble protien)
Insect mortality (%)
Leaf Fruit
Control 0.00 0 0
Bt1 0.26 + 0.07 80 50
Bt2 0.10 + 0.03 100 100
Bt3 0.11 + 0.03 100 100
Bt4 0.04 + 0.005 100 100
Bt5 0.11 + 0.04 60 80
Bt6 0.42 + 0.09 100 100
Bt7 0.60 + 0.05 100 100
Experimental details:
Bacterial strain used : A. tumefaciens LBA 4402
Variety used : Italian tomato genotype LEPA
Explant : Cotyledonary leaves from 10-day old seedlings
Media (5.7 pH) : ½ MS + Sucrose (1%) + Agar (0.8%)
Gene : cry1Ab gene
01/01/2014 SAMI 45
Tomato expressing Cry1A(b) insecticidal protein protected
against tomato fruit borer, damage in the laboratory and
green house
Harish Kumar*, Vinod Kumar, 2003, Gurgaon
01/01/2014 SAMI 46
Plate 4: Damage caused by H. armigera to the fruit of non-transgenic and
transgenic tomato plants in the laboratory.
Harish Kumar*, Vinod Kumar, 2003, Gurgaon
01/01/2014 SAMI 47
Harish Kumar*, Vinod Kumar, 2003, Gurgaon
Plate 5: Extent of damage caused by larvae of H. armigera to transgenic Bt and
non transgenic tomato plants in the green house
Genetic manipulation for disease tolerance
01/01/2014 SAMI 48
01/01/2014 SAMI 49
Experimental details-
Bacterial strain used : A. tumefaciens SRC 1102
Explant : young leaf discs
Gene : Pn-AMPs
Source : Pharbitis nil
Hevein-like proteins from pharbitis nil confers disease
resistance against phytopathogenic fungi in tomato
Lee et al, 2003
Figure 7: Physical map of binary vector Pn-AMP2643
used for transformation
01/01/2014 SAMI 50
Lee et al., 2003
Plate 6: Transgenic tomato conforming resistance against F. oxysporum
transformed with pnAMPs gene.
01/01/2014 SAMI 51
Lee et al., 2003
Evaluation of transgenic Tomato plants against CMV strain
WL under field conditions
01/01/2014 SAMI 52
Fuchs et al., 1996, Geneva
Experimental details-
Bacterial strain used : A. tumefaciens strain C58Z707
Variety used : TT5-007-11, TT5-007-11 x Solarset (Hy)
Explant : 7 day old cotyledon sections (0.2 x 0.5 cm)
Media (5.7 pH) : MS + B5 Vit + BA (2.5 mg/l) + IAA (1.0 mg/l) +
Agar (0.8 %)
Gene : CMV-WL CP gene
Table 11: Evaluation of transgenic tomato lines for resistance
under field conditions
(Fuchs et al., 1996)
01/01/2014 SAMI 53
Lines/hybrids Infected/tested Infection (%)
Transgenic homozygous
TT5-007-11
0/176 0
Control G80 65/176 37
Transgenic TT5-007-11 X
Solarset hybrid
0/22 0
Control solarset 17/22 77
Plate 7: Disease reactions TT5-007-11 and G-80
(Fuchs et al., 1996)
01/01/2014 SAMI 54
Table 12: Performance of transformed and non-
transformed lines
(Fuchs et al., 1996)
01/01/2014 SAMI 55
Line No. of
plants
tested
Average
Plant
height
Plants
with
fruits
(%)
Average
No. of
fruits/plant
Average
Yield
(g)/plant
Average
Fruit
wieght
(g)
Transgenic
TT5-007-11
176 64 + 12 92 19 +11 1840 97
Non transformed
G-80
65 47 + 11 56 2 + 3 108 54
Virus Method Workers
Spotted wilt
virus
RNA mediated Goldbatch et al. (2003)
Yellow leaf curl Rep Protein
Brunetti et al. (1997); Antignus
et al. (2007)
Goldenn
mosaic virus
Sense and
antisense RNA
Day et al. (1991)
TMV
N gene from
Tobacco
Whitham et al. (1996)
Bushy Stunt
Virus
ScFvs Boonrod et al. (2000)
Table 13: Reports on development of transgenic tomato
plants for virus resistance
(Prins et al., 2007)
01/01/2014 SAMI 56
Genetic manipulation for abiotic stress
tolerance
01/01/2014 SAMI 57
LeERF1 improves tolerance to drought in
Tomato
01/01/2014 SAMI 58
Lu et al., 2010, Beijing
Experimental details:
Variety used : Zhongshu No.4
Explant : 7 day old cotyledon sections (0.2 x 0.5 cm)
Gene : LeERF1 gene
Plate 8: Evaluation of drought tolerance in 4 week old seedlings
by withholding water for 10 days
Control
Drought
stress
Non-
transfered
Sense
LeERF1
Antisense
LeERF1
(Lu et al., 2010)01/01/2014 SAMI 59
(Lu et al., 2010)
Figure 9: proline content on water stress
01/01/2014 SAMI 60
01/01/2014 SAMI 61
Experimental details:
Bacterial strain used : A. tumefaciens
Variety used : Micro tom
Explant : 7 day old cotyledon
Gene : betaine aldehyde dehydrogenase
(BADH) gene,
Salt-inducible expression of SIBADH gene in transgenic
tomato enhances salt tolerance
Wang et al, 2013
01/01/2014 SAMI 62
(A) Under the non-stress condition (B) After 7 days of salt
stress by treatment with 200 mM NaCl,
Wang et al, 2013
Genetic manipulation for quality
improvement
01/01/2014 SAMI 63
Suppression of ACC oxidase expression in
Tomato using heterologus gene from Banana
01/01/2014 SAMI 64
Batra et al., 2010, Lucknow
Experimental details:
Variety used : Ailsa craig
Explants : Cotyledons
Source of gene : Banana
Gene : MaCO gene
Method : Particle bombardment
Plate 10: On vine (a) and post harvest (b) developmental stages of non-
transformed and transformed tomatoes
a
b
(Batra et al., 2010)01/01/2014 SAMI 65
The ‘FLAVR SAVR
TM
’ affair
 First GM whole food to be sold in public market
 FDA approved on 18 May, 1994 & sale begun on 21st
May
 Technology: Antisense RNA to regulate the
expression of polygalacturunase (PG)
 Developed by Calgene company, Davis, California
01/01/2014 SAMI 66
‘FLAVR SAVR
TM
’ Contd..
 Stay ‘ripe’ but ‘not rot’
 For 10 days
 No refrigeration needed
01/01/2014 SAMI 67
Table 14: Comparison between FLAVR SAVR and control
line for nutritional values
01/01/2014 SAMI 68
Transgenic Tomato Researches in India
01/01/2014 SAMI 69
Trait Gene Stage
Year of
completion
Salinity, Drought, Cold
ect.
Mannitol-1-phospate
dehydrogenase
T4 2014
Shelf life Arginine decarboxylase T3 2014
Male sterility i-Ornithine decarboxylase T3 2015
Salinity Glyoxalsae I & II T3 2015
Fungus, Nematode i-Ornithine decarboxylase T3 2015
Fungus, Nematode i-Chitin synthase T3 2015
Fungus Afp-ca T3 2015
Rakesh, 2012
Table 15: List of on-going transgenic work in India through
ICAR
01/01/2014 SAMI 70
Regulatory bodies in India
1. Institutional Biosafety Committees (IBSC)
2. Recombinant DNA Advisory Committee (RDAC)
3. Review Committee on Genetic Manipulation (RCGM)
4. Genetic Engineering Approval Committee (GEAC)
5. State Biosafety Coordination Committees (SBCC)
01/01/2014 SAMI 71
Some news clippings
01/01/2014 SAMI 72
Take home message
01/01/2014 SAMI 73
SAFETY: GM foods and crops are as safe
as conventional ones
REGULATION: Highly regulated. Approval
process requires many tests and years
ENVIRONMENT: Their is no evidence
01/01/2014 SAMI 74
ENVIRONMENTAL BENEFITS: Require
less pesticides, less tillage.
BETTER NUTRITION: futuristic GM crops
FARMERS: want GM crops because crop
production is cheaper.
OPPONENTS OF GM CROPS: have not
brought forth scientific evidence to backup
their claims.
Conventional breeding for traits
is unpredictable
Use of biotech tools will allow us
to go from unpredictable to
predictable engineering
01/01/2014 SAMI 75
01/01/2014 SAMI 76

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Transgenics - a biotech approach for improvement of tomato (tomato breeding)

  • 2. UNIVERSITY OF AGRICULTURAL AND HORTICULTURAL SCIENCES, SHIMOGA. COLLEGE OF HORTICULTURE, MUDIGERE.
  • 3.  Introduction  Transformation methods  Practical application  Herbicidal, Pest, Disease, Drought – Tolerance, and Quality  Indian research  Conclusion 01/01/2014 SAMI 3
  • 4. Introduction 01/01/2014 SAMI 4 Biotechnology is one of the tools , but a potentially important one, in the struggle to reduce poverty, improve food security, reduce malnutrition and improve livelihood of the rural and the urban poor. - Persley, 1999
  • 5.  Modification of an organism’s DNA in order to achieve a desired trait. 01/01/2014 SAMI 5 What are genetically modified organisms (GMO) ? + = Arctic fish DNA Tomato A tomato resistant to frost What is transgenic? http://en.wikipedia.org/wiki/Fish_tomato
  • 6. 01/01/2014 SAMI 6 Brief history of transgenics ISAAA, 2011 1985 1st transgenic plants produced. 1994 Flavr-Savr tomato is released 1996 Herbicide- and insect- resistant crops approved for cultivation 2000 Golden rice with ß-carotene developed 2011 160 million ha. of GM crops planted. GM crops considered substantially equivalent to hybrid varieties 1992
  • 7. 01/01/2014 SAMI 7 How transgenic breeding differs from conventional breeding?
  • 8. Conventional Breeding Transgenesis Current cultivar Wild relative GOI Unwanted genes Back cross F1 generation F2 generation Many backcrosses New Cultivar Unwanted Genes GOI Current Cultivar Transfer in to plasmid agrobacterium GOI Genes required for transfer & marker genes New Cultivar Unrelated organism Genes required for transfer & marker genes GOI 01/01/2014 SAMI 8
  • 9. TOMATO • Most common vegetable • Indian meals incomplete without tomato. • Botanical name Solanum lycopersicum L. • Chromosome number 2n = 24 • Well distributed throughout the world • One among the top five vegetables 01/01/2014 SAMI 9 Area Production Productivity(t/ha) INDIA 8.65 lakh ha. 16.82 lakh tons 19.5 KARNATAKA 51.2 thousand ha. 1756.7 thousand tons 19.5 Anon 2012
  • 10. Source – NBPGR, NCBI etc., Vector Construction – Plasmid, cosmid, bacteriphage, virus etc., Transformations – Microinjection, Gene gun, Electrophoretion, Agrobacterium, etc., Selection of transgenic plant (Antibiotic containing media) Elimination of marker and backbone (through DEX media) Confirmation (through PCR) Expression – Southern blotting, RT PCR, ELISA 01/01/2014 SAMI 10
  • 12. Microinjection Biolistics - gene gun/ particle bombardment Electroporation Silicon carbide fibers PEG DEAE-dextran Calcium phosphate A. tumefaciens A. rhizogenes Virus-mediated Pollen transformation Meristem transformation Singh B. D., 2009 01/01/2014 SAMI 12 Methods of plant transformation PHYSICAL CHEMICAL BIOLOGICAL IN PLANTA
  • 13. Agrobacterium mediated transformation • Most extensively used method • Natural ability of Agrobacterium to transfer plants • First report: McCormick et al.(1986) • Cotyledons/leaves are used for transformation • A. tumefaciens and A. rhizogenes 01/01/2014 SAMI 13
  • 14. Tomato transformation mediated by Agrobacterium 01/01/2014 SAMI 14
  • 16. Simple and efficient Agrobacterium mediated procedure for transformation of Tomato 01/01/2014 SAMI 16 Bacterial strain used : A. tumefaciens strain AGL 1 Growth conditions- Growth room temperature : 28 10C Culturing of Agrobacterium : Rotary shaker (280C) for 72hrs at 200 rpm Explants : Cotyledons from 10 day old plants Size of explant : 0.7 cm x 1.0 cm Varieties studied : Pusa Ruby, Arka Vikas and Sioux Sharma et al., 2009, New Delhi
  • 17. Figure 1 : Vectors used for transformation of Tomato using A. tumefaciens strain AGL 1 (Sharma et al., 2009) 01/01/2014 SAMI 17
  • 18. Plate 1: Different stages of Solanum lycopersicum var. Pusa Ruby transformation 01/01/2014 SAMI 18 (Sharma et al., 2009)
  • 19. Table 1: Effect of bacterial concentration and co-cultivation period on transformation of Pusa Ruby (Sharma et al., 2009) 01/01/2014 SAMI 19 Bacterial concentration No. of explants Averaga percent transformation efficeincy + SE 72 h cocultivation 96 h cocultivation 0.5 X 108 70 20.7 + 1.01 22.1 + 1.01 1.0 X 108 70 41.4 + 2.02 24.3 + 2.02 2.0 X 108 70 38.6 + 2.02 19.3 + 3.03 5.0 X 108 70 36.4 + 1.01 17.9 + 1.01 10 X 108 70 12.9 + 2.02 -
  • 20. Table 2: Transformation efficiency of different Tomato varieties using optimized protocol (Sharma et al., 2009) 01/01/2014 SAMI 20 Vector used Tomato variety Average No. of explants co- cultivated Average transformation efficiency (% + SE) pCTBE2L Pusa Ruby 174 40.5 + 0.80 pRINASE2L Pusa Ruby 163 41.1 + 0.89 pCTBE2L Sioux 150 41.0 + 1.00 pCTBE2L Arka Vikas 150 22.0 + 1.50
  • 21. Biolistic gun • Most successfully applied • Also known as ‘Particle bumbardment’ • Principle: High velocity discharge of DNA ‘bullets’ coated with gold or nickel particles • Non specificity of species • Gene integration is random • Low rate of stable transformation (10-5) 01/01/2014 SAMI 21
  • 22. Plate 2 : Gene gun 01/01/2014 SAMI 22
  • 25. Tomato transformation using biolistic gun • Intoduced gene : β glucuronidase (gusA) • Genotype : IPA-3 • Explants : Shoot tips, hypocotyls and cotyledon • Particle gun used : Bio-Rad Gun • TC media : MS + BAP (2.0 mg/l) + Kinetin (1.0 mg/l) 01/01/2014 SAMI 25 Ruma et al., 2009, Ludhiana
  • 26. Source df Mean sum of squares Target distance DNA quantity Pre- bumbardment culture Post- bumbardment culture Explant 2 210.71* 9.66 45.29* 8.24* Parameters 3 1457.75* 1508.98* 772.85* 548.94* Explant x Parameters 6 37.12* 52.72* 1207.10* 3.21 Error 24 7.04 14.78 12.25 26.42 Table 3 : ANOVA for GUS expression as affected by different parameters of particle gun (Ruma et al., 2009) Figure 2: Effect of target distance on transformation 01/01/2014 SAMI 26
  • 27. Source df Mean sum of squares Target distance DNA quantity Pre- bumbardment culture Post- bumbardment culture Explant 2 210.71* 9.66 45.29* 8.24* Parameters 3 1457.75* 1508.98* 772.85* 548.94* Explant x Parameters 6 37.12* 52.72* 1207.10* 3.21 Error 24 7.04 14.78 12.25 26.42 Table 4: ANOVA for GUS expression as affected by different parameters of particle gun (Ruma et al., 2009) Figure 3: Effect of DNA quantity on transformation 01/01/2014 27SAMI
  • 28. Source df Mean sum of squares Target distance DNA quantity Pre- bumbardment culture Post- bumbardment culture Explant 2 210.71* 9.66 45.29* 8.24* Parameters 3 1457.75* 1508.98* 772.85* 548.94* Explant x Parameters 6 37.12* 52.72* 1207.10* 3.21 Error 24 7.04 14.78 12.25 26.42 Table 5: ANOVA for GUS expression as affected by different parameters of particle gun (Ruma et al., 2009) Figure 4: Effect of pre-bumbardment culture on transformation 01/01/2014 SAMI 28
  • 29. Source df Mean sum of squares Target distance DNA quantity Pre- bumbardment culture Post- bumbardment culture Explant 2 210.71* 9.66 45.29* 8.24* Parameters 3 1457.75* 1508.98* 772.85* 548.94* Explant x Parameters 6 37.12* 52.72* 1207.10* 3.21 Error 24 7.04 14.78 12.25 26.42 Table 6: ANOVA for GUS expression as affected by different parameters of particle gun (Ruma et al., 2009) Figure 5: Effect of post bumbardment culture on transformation 01/01/2014 SAMI 29
  • 30. Plate 2: Different explants showing GUS expresion a. Cotyledons, b. Shoot tips, c. Hypocotyls, d. Leaf, e. Callus, f. Root like structures 01/01/2014 SAMI 30
  • 31. Pollen mediated transformation of Tomato 01/01/2014 SAMI 31
  • 32. 01/01/2014 SAMI 32 Does not require tissue culture and plant regeneration Produces genetically uniform progeny Not expensive Genotype independent – monocots/dicots Utilizes normal fertilization process Benefits of pollen transformation
  • 33. 01/01/2014 SAMI 33 Bacterial strain used: A. tumefaciens strain LBA4404 Growth conditions: Growth room temperature : 28 ± 10C Culturing medium : Yeast Extract Mannitol Agar + Streptomycin (100 µg/ml) + Rifampicin (25 µg/ml) + Kanamycin (50 µg/ml) In vitro manipulation of pollen for transformation in Tomato Satish, 2009, Dharwad
  • 34. (Satish, 2009) 01/01/2014 SAMI 34 Plate 3: Vector used for transformation of pollen of Tomato
  • 35. 01/01/2014 SAMI 35 Table 7: In vitro pollen germination medium for Tomato (Pusa Ruby) (Satish, 2009) Medium Germination (%) Tube length (m) PGM-1 32.00c 190c PGM-2 46.80b 213b PGM-3 92.96a 281a CD @1% 1.62 1.00 Media constitution: PGM-1: Sucrose (18%) + Agarose (1%) + Boric acid (0.015%) PGM-2: Sucrose (16%) + Boric acid (0.6mM) + CaNO3 (0.8mM) + MgSO4 (0.5mM) PGM-3: Sucrose (10%) + Boric acid (100mg/l) +GA (125µM)
  • 37. Herbicidal tolerance Pest tolerance Disease tolerance Abiotic stress tolerance Quality improvement 01/01/2014 SAMI 37
  • 38. Engineering herbicidal resistance in plants by expression of detoxifying enzyme 01/01/2014 SAMI 38 Block et al., 2007, England Experimental details: Bacterial strain used : A. tumefaciens strain C58C1 Rif Variety used : Petit Havana Explant : Leaf disc Media (5.7 pH) : ½ MS + Sucrose (1%) + Agar (0.8%) Gene : bar gene Mechanism : PAT (Phosphinothricin acetyltransferace) detoxification
  • 39. Figure 6: Ammonia determination (% basal NH4 + content) after spraying Basta® (20 l/ha) (Block et al., 2007) 01/01/2014 SAMI 39
  • 40. Class of herbicide Compound/ Herbicide Transgene/ Mechanism Company Phosphonic acid Phoshanothricin (Basta® , Liberty® ) bar gene/ PAT detoxification Syngenta Sulphonylurea Chlorosulphuron (Glean® ) Mutant plant/ acetolactate synthase Dupont- Poineer-Hi- Bred Nitriles Bromoxynil (Buctril® ) Nitrilase detoxification Calgene/ Bayer crop science (Slater, 2010) 01/01/2014 SAMI 40
  • 41. Genetic manipulation for pest tolerance 01/01/2014 SAMI 41
  • 42. table 9: Different versions of the Cry genes effective against different orders of insects Cry gene designation Toxic to these insect orders CryIA(a), CryIA(b), CryIA(c) Lepidoptera Cry1B, Cry1C, Cry1D Lepidoptera CryII Lepidoptera, Diptera CryIII Coleoptera CryIV Diptera CryV Lepidoptera, Coleoptera 01/01/2014 SAMI 42 Byrne et al., 2002
  • 43. Experimental details: Bacterial strain used : A. tumefaciens strain LBA 4404 Variety used : Pusa Ruby Explant : Cotyledonary leaves from 10-day old seedlings Media (5.7 pH) : ½ MS + Sucrose (1%) + Agar (0.8%) Gene : cry1Ac gene 01/01/2014 SAMI 43 Transgenic tomato plants resistant to fruit borer (Helicoverpa armigera Hubner) Mandaokar et al., 2000, New Delhi
  • 44. 01/01/2014 SAMI 44 Mandaokar et al., 2000, New Delhi Table 10: Expression of Cry 1 Ac protein in transformed Pusa Ruby Plant no. Cry1Ac content(% of total soluble protien) Insect mortality (%) Leaf Fruit Control 0.00 0 0 Bt1 0.26 + 0.07 80 50 Bt2 0.10 + 0.03 100 100 Bt3 0.11 + 0.03 100 100 Bt4 0.04 + 0.005 100 100 Bt5 0.11 + 0.04 60 80 Bt6 0.42 + 0.09 100 100 Bt7 0.60 + 0.05 100 100
  • 45. Experimental details: Bacterial strain used : A. tumefaciens LBA 4402 Variety used : Italian tomato genotype LEPA Explant : Cotyledonary leaves from 10-day old seedlings Media (5.7 pH) : ½ MS + Sucrose (1%) + Agar (0.8%) Gene : cry1Ab gene 01/01/2014 SAMI 45 Tomato expressing Cry1A(b) insecticidal protein protected against tomato fruit borer, damage in the laboratory and green house Harish Kumar*, Vinod Kumar, 2003, Gurgaon
  • 46. 01/01/2014 SAMI 46 Plate 4: Damage caused by H. armigera to the fruit of non-transgenic and transgenic tomato plants in the laboratory. Harish Kumar*, Vinod Kumar, 2003, Gurgaon
  • 47. 01/01/2014 SAMI 47 Harish Kumar*, Vinod Kumar, 2003, Gurgaon Plate 5: Extent of damage caused by larvae of H. armigera to transgenic Bt and non transgenic tomato plants in the green house
  • 48. Genetic manipulation for disease tolerance 01/01/2014 SAMI 48
  • 49. 01/01/2014 SAMI 49 Experimental details- Bacterial strain used : A. tumefaciens SRC 1102 Explant : young leaf discs Gene : Pn-AMPs Source : Pharbitis nil Hevein-like proteins from pharbitis nil confers disease resistance against phytopathogenic fungi in tomato Lee et al, 2003
  • 50. Figure 7: Physical map of binary vector Pn-AMP2643 used for transformation 01/01/2014 SAMI 50 Lee et al., 2003
  • 51. Plate 6: Transgenic tomato conforming resistance against F. oxysporum transformed with pnAMPs gene. 01/01/2014 SAMI 51 Lee et al., 2003
  • 52. Evaluation of transgenic Tomato plants against CMV strain WL under field conditions 01/01/2014 SAMI 52 Fuchs et al., 1996, Geneva Experimental details- Bacterial strain used : A. tumefaciens strain C58Z707 Variety used : TT5-007-11, TT5-007-11 x Solarset (Hy) Explant : 7 day old cotyledon sections (0.2 x 0.5 cm) Media (5.7 pH) : MS + B5 Vit + BA (2.5 mg/l) + IAA (1.0 mg/l) + Agar (0.8 %) Gene : CMV-WL CP gene
  • 53. Table 11: Evaluation of transgenic tomato lines for resistance under field conditions (Fuchs et al., 1996) 01/01/2014 SAMI 53 Lines/hybrids Infected/tested Infection (%) Transgenic homozygous TT5-007-11 0/176 0 Control G80 65/176 37 Transgenic TT5-007-11 X Solarset hybrid 0/22 0 Control solarset 17/22 77
  • 54. Plate 7: Disease reactions TT5-007-11 and G-80 (Fuchs et al., 1996) 01/01/2014 SAMI 54
  • 55. Table 12: Performance of transformed and non- transformed lines (Fuchs et al., 1996) 01/01/2014 SAMI 55 Line No. of plants tested Average Plant height Plants with fruits (%) Average No. of fruits/plant Average Yield (g)/plant Average Fruit wieght (g) Transgenic TT5-007-11 176 64 + 12 92 19 +11 1840 97 Non transformed G-80 65 47 + 11 56 2 + 3 108 54
  • 56. Virus Method Workers Spotted wilt virus RNA mediated Goldbatch et al. (2003) Yellow leaf curl Rep Protein Brunetti et al. (1997); Antignus et al. (2007) Goldenn mosaic virus Sense and antisense RNA Day et al. (1991) TMV N gene from Tobacco Whitham et al. (1996) Bushy Stunt Virus ScFvs Boonrod et al. (2000) Table 13: Reports on development of transgenic tomato plants for virus resistance (Prins et al., 2007) 01/01/2014 SAMI 56
  • 57. Genetic manipulation for abiotic stress tolerance 01/01/2014 SAMI 57
  • 58. LeERF1 improves tolerance to drought in Tomato 01/01/2014 SAMI 58 Lu et al., 2010, Beijing Experimental details: Variety used : Zhongshu No.4 Explant : 7 day old cotyledon sections (0.2 x 0.5 cm) Gene : LeERF1 gene
  • 59. Plate 8: Evaluation of drought tolerance in 4 week old seedlings by withholding water for 10 days Control Drought stress Non- transfered Sense LeERF1 Antisense LeERF1 (Lu et al., 2010)01/01/2014 SAMI 59
  • 60. (Lu et al., 2010) Figure 9: proline content on water stress 01/01/2014 SAMI 60
  • 61. 01/01/2014 SAMI 61 Experimental details: Bacterial strain used : A. tumefaciens Variety used : Micro tom Explant : 7 day old cotyledon Gene : betaine aldehyde dehydrogenase (BADH) gene, Salt-inducible expression of SIBADH gene in transgenic tomato enhances salt tolerance Wang et al, 2013
  • 62. 01/01/2014 SAMI 62 (A) Under the non-stress condition (B) After 7 days of salt stress by treatment with 200 mM NaCl, Wang et al, 2013
  • 63. Genetic manipulation for quality improvement 01/01/2014 SAMI 63
  • 64. Suppression of ACC oxidase expression in Tomato using heterologus gene from Banana 01/01/2014 SAMI 64 Batra et al., 2010, Lucknow Experimental details: Variety used : Ailsa craig Explants : Cotyledons Source of gene : Banana Gene : MaCO gene Method : Particle bombardment
  • 65. Plate 10: On vine (a) and post harvest (b) developmental stages of non- transformed and transformed tomatoes a b (Batra et al., 2010)01/01/2014 SAMI 65
  • 66. The ‘FLAVR SAVR TM ’ affair  First GM whole food to be sold in public market  FDA approved on 18 May, 1994 & sale begun on 21st May  Technology: Antisense RNA to regulate the expression of polygalacturunase (PG)  Developed by Calgene company, Davis, California 01/01/2014 SAMI 66
  • 67. ‘FLAVR SAVR TM ’ Contd..  Stay ‘ripe’ but ‘not rot’  For 10 days  No refrigeration needed 01/01/2014 SAMI 67
  • 68. Table 14: Comparison between FLAVR SAVR and control line for nutritional values 01/01/2014 SAMI 68
  • 69. Transgenic Tomato Researches in India 01/01/2014 SAMI 69
  • 70. Trait Gene Stage Year of completion Salinity, Drought, Cold ect. Mannitol-1-phospate dehydrogenase T4 2014 Shelf life Arginine decarboxylase T3 2014 Male sterility i-Ornithine decarboxylase T3 2015 Salinity Glyoxalsae I & II T3 2015 Fungus, Nematode i-Ornithine decarboxylase T3 2015 Fungus, Nematode i-Chitin synthase T3 2015 Fungus Afp-ca T3 2015 Rakesh, 2012 Table 15: List of on-going transgenic work in India through ICAR 01/01/2014 SAMI 70
  • 71. Regulatory bodies in India 1. Institutional Biosafety Committees (IBSC) 2. Recombinant DNA Advisory Committee (RDAC) 3. Review Committee on Genetic Manipulation (RCGM) 4. Genetic Engineering Approval Committee (GEAC) 5. State Biosafety Coordination Committees (SBCC) 01/01/2014 SAMI 71
  • 73. Take home message 01/01/2014 SAMI 73 SAFETY: GM foods and crops are as safe as conventional ones REGULATION: Highly regulated. Approval process requires many tests and years ENVIRONMENT: Their is no evidence
  • 74. 01/01/2014 SAMI 74 ENVIRONMENTAL BENEFITS: Require less pesticides, less tillage. BETTER NUTRITION: futuristic GM crops FARMERS: want GM crops because crop production is cheaper. OPPONENTS OF GM CROPS: have not brought forth scientific evidence to backup their claims.
  • 75. Conventional breeding for traits is unpredictable Use of biotech tools will allow us to go from unpredictable to predictable engineering 01/01/2014 SAMI 75