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The application of genetic transformation at ARC-VOPI to improve plant traits Dr. Inge Gazendam Regional Plant biotechnology forum 30 October 2014 ARC-Roodeplaat, Vegetable and Ornamental Plant Institute, Pretoria
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Page 1: The application of genetic transformation at ARC -VOPI to ...Tomato Melon Tolerance to: Fungus Virus Insects (PTM) Drought Herbicide Delayed ripening GUS PGIP, Peroxidase PLRV, PVY,

The application of genetic transformation at ARC-VOPI

to improve plant traits

Dr. Inge Gazendam Regional Plant biotechnology forum

30 October 2014 ARC-Roodeplaat, Vegetable and Ornamental Plant Institute, Pretoria

Page 2: The application of genetic transformation at ARC -VOPI to ...Tomato Melon Tolerance to: Fungus Virus Insects (PTM) Drought Herbicide Delayed ripening GUS PGIP, Peroxidase PLRV, PVY,

Overview • Background • History of projects at the institute • Recent projects

– Virus tolerant Ornithogalum – Drought tolerant potato

• Personal comments

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Background • Discovery of tumor inducing principle in Agrobacterium

– Smith and Townsend 1907

• Ti plasmid development – Schell 1974

• Application on model system A. thaliana – Somerville 1994

• Requirements – Tissue culture – Genes – Methods of transfer

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Biolistics

DNA adhered to tungsten/gold particles

Particle inflow gun

Target tissue: Callus, embryos, meristems,

cell suspensions

GUS staining of transformed cells

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Agrobacterium Target tissue: wounded explant Cut into small pieces & pre-culture

Plant regeneration

Infect with Agrobacterium

= co-culture stage

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History of projects Crops Traits Genes

Tobacco Potato Ornithogalum Soybean A. thaliana Sweetpotato Tomato Melon

Tolerance to: Fungus Virus Insects (PTM) Drought Herbicide Delayed ripening

GUS PGIP, Peroxidase PLRV, PVY, TSWV, SPFM, OrMV CryIa1 (Bt) LEA5, P5CR, SOD BASTA Inducible promoters: lupin, GST1

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Recent projects • Drought tolerant potato • Virus tolerant Ornithogalum

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A transgenic approach to improve the drought tolerance of potato

Page 9: The application of genetic transformation at ARC -VOPI to ...Tomato Melon Tolerance to: Fungus Virus Insects (PTM) Drought Herbicide Delayed ripening GUS PGIP, Peroxidase PLRV, PVY,

Objective • Create a more drought tolerant potato through genetic

transformation – Enhance the transcription of drought-protective genes – Use potato’s own TF gene (StMYB1R-1) – Cis-genic approach more readily accepted

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Strategy

rd29A promoter StMYB1R-1 TF gene

Stress-inducible promoter

Transcription factor gene

Gene 1

Gene 2

Gene 3

Gene 4

Gene …

Downstream drought protective genes

activate

activate Desiccation stress

A. thaliana S. tuberosum

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Methodology 1. Gene isolation and cloning 2. Plant transformation 3. Molecular characterisation

1. PCR 2. GUS activity assays 3. RT-qPCR 4. Southern blot

4. Greenhouse drought trial

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1. Gene isolation and cloning

RT-PCR BP1 potato

PCR A. thaliana

StMYB1R-1 rd29A prom

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Plant transformation constructs A

pBI121

B

pBI121-rd29Ap:GUS

C

pBI121-CaMV:StMYB1R-1

D

pBI121-rd29Ap:StMYB1R-1

E

pBI121-neg

rd29Ap

StMYB1R-1

CaMV 35S GUS

rd29Ap StMYB1R-1

CaMV 35S

GUS

GUS

1. Gene isolation and cloning

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2. Plant transformation

Transform BP1 potato by Agrobacterium infection A:Transformed stem explants on selective medium B: Regeneration of shoots from transformed potato callus C: Shoots transferred into rooting medium

A B C

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3. Molecular analysis PCR with 6 different primer combinations • StMYB1R-1, rd29Ap, GUS, vector-specific • 92 plants selected for genomic DNA isolations • 83 lines were found to contain the expected inserted genes

M + 13 14 15 16 17 18 19 20 21 22 23 24

M + 1 2 3 4 5 6 7 8 9 10 11 12 Constructs Correct genes

A CaMV prom GUS vector 10 9

B rd29A prom GUS vector 24 24

C CaMV prom StMYB1R-1 vector 24 19

D rd29A prom StMYB1R-1 vector 24 21

E - GUS vector 10 10

92 83

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3. Molecular analysis

D: rd29Ap:StMYB1R-1

Transgenic StMYB1R-1 expression levels D lines: inducible transgenic StMYB1R-1 expression

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2 5 2 1 4 3 2 1 1 3 2 7 copies

M BP1 C2 C3 C9 C11 C16 C22 BP1 M BP1 D6 D16 D18 D19 D21 D23 BP1 +1 10 copies + 1 10 copies

C: CaMV:StMYB1R-1 D: rd29Ap:StMYB1R-1

904 bp

Southern blot of 12 selected lines

3. Molecular analysis

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4. Greenhouse drought trial • Measure:

a) Relative water content (RWC) b) Visual appearance c) Survival after drought stress d) Yield of biomass (tubers & leaves)

Control Stress 8 dwow

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4. Greenhouse drought trial Visual appearance – Trial 1 • Foliar tissue drooping after 11 days

BP1 C3 D6 BP1 C3 D6

Stress Control

One representative of each line

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Results • Greenhouse trials for improved drought tolerance

– First greenhouse trial: • Three transgenic lines (D6, C3 and D16) perform better under drought

stress than wild-type BP1 • RWC, visual appearance and survival

– Second greenhouse trial: • Confirm RWC% results for only line D6 • Biomass yield difference under drought (fresh and dried leaf and

tubers) between transgenic lines and BP1 was not significant

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Conclusion • Successfully transformed a local cultivar (BP1) with

a potato TF gene – Enhance the transcription of drought-protective genes – Stable insertion into genome and expression of transcript

• Greenhouse trials for evaluating improved drought tolerance – Differences in responses between transgenic lines and ‘BP1’

under drought conditions was not significant

• Same strategy not necessarily successful when applied to different organism and using other gene

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Transformation of Ornithogalum

for virus resistance

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Background: Ornithogalum • Indigenous flower species • Popular for pot plants and cut flowers • Important for the South African flower industry • Problem: highly susceptible to viruses, especially

Ornithogalum mosaic virus (OrMV)

Virus symptoms on leaves Yellow flower of Ornithogalum hybrid A2

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Objective • The release of a transgenic Ornithogalum line with

effective resistance against OrMV • Benefit:

– Economic benefit to the South African cut flower industry

– Use this line to incorporate virus resistance into other susceptible Ornithogalum varieties in a breeding program

– Reduce yield losses of growers – Yield products of higher quality

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Methods • OrMV coat protein and OrMV replicase genes • Virus resistance through gene silencing (RNAi)

– Post-transcriptional silencing (PTGS) – Use OrMV coat protein gene to silence virus gene – Self-complementary hairpin RNA (hpRNA)

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Methods • Gene synthesis and cloning

– Coat protein gene of a South African isolate of OrMV

– Add two pairs of restriction sites during PCR

– pSTARLING-A vector from CSIRO • Commonwealth Scientific and Industrial

Research Organisation, Australia

pSTARLING Hairpin7521 bp

cre introntmL terminatorM13F(-20)

T7 primer

Ubi prom & intro

Amp resistance

OMVCP

OMVCP

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Methods • pCAMBIA1300 plant

transformation vector

• Agrobacterium-mediated transformation – leaf explants of Ornithogalum A2 – Regenerate putative transgenic plants from transformed callus – Hygromycin antibiotic selection

pCAM1300-RNAi OMVCP A13619 bp

kanamycin R

Hygromycin R

cre intron

CaMV 3'UTR (polyA signal)

pVS1 Sta

pBR322 bom site

T border (L)

T border (R)tmL terminator

Ubi prom & intron

CaMV35S

PlacZ

pVS1-REP

pBR322 ori

OMVCP

OMVCP

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Results Callus

Root Excise

Shoots

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Results • PCR screening with OrMV-CP primers

– 18 lines positive out of 20 screened

PCR screen results with OrMV-CP specific primers pl+: positive plasmid control pC: pCAMBIA1300 transgenic A2: Untransformed Ornithogalum line A2 - : Negative water control

M pl+ 1 2 3 4 5 6 7 8 9 10 pC A2 - M

M pl+ 11 12 13 14 15 16 17 18 19 20 pC A2 - M

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Results • Multiplication of the selected transgenic lines

– Between 37 and 154 in vitro plantlets each of 18 individual transgenic lines

Transgenic Ornithogalum plants that are being multiplied in vitro in tubs

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Greenhouse efficacy trials • Require pure OrMV source for virus infection trials

– Screen diseased plants from flower breeding program with RT-PCR – Electron microscopy of virus-infected plant samples – Sequencing of cloned coat protein RT-PCR products

• Mechanical infection method – Very low transmission rates – Symptoms visible only after 8 weeks

Virus symptoms on infected Ornithogalum plant

OrMV successfully transmitted to only 2 out of 30 healthy plants

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Greenhouse efficacy trials • Greenhouse trial planted on 30 July 2014

– 24 replicates of each transgenic line – Ready for infection as soon as successful infection method is

identified – Establishment rate 2 months later = 97%

Hardening off in vitro transgenic Ornithogalum

plants

Transgenic Ornithogalum plants after 2 months in the

greenhouse

Dripper irrigated pots before planting

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Way forward To perform virus resistance efficacy trial: Multiplied 18 transgenic events in vitro Yes Have OrMV source Yes Mechanical infection method Optimise

After virus infection: Track progression of infection with ELISA and visual assessments

Pending

Molecular characterisation of transgenic lines: gDNA isolation without polysaccharides Optimise Southern blot to verify stable integration of OrMV-CP DNA into plant genome

Pending

Northern blots of siRNA expression levels Pending

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Personal comments 29th International Horticultural Congress (IHC2014), 17-22 August 2014, Brisbane, Australia

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Personal comments • Regulatory issues • Red zone: deregulation and commercialization

– Scientists out of their comfort zone – Don’t get anywhere if you listen to what you hear

• Dennis Gonsalves

• Refine technology = new plant breeding techniques – Site-directed nucleases (SDN)

• Introduce foreign stretch of DNA into specific site – Oligonucleotide directed mutagenesis (ODM)

• Repair mismatched oligonucleotide = single mutation at defined site – Genome editing

• TALENs (Transcription activator-like effector nuclease) • CRISPR-Cas (Clustered regularly interspaced palindromic repeat associated proteins)

– Regulatory considerations = GMO or not? – Regulate product and not technology that produced it

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Personal comments • 1st generation GMO was to producer benefit • Good examples

– Bt toxin, little collateral damage • Alternative to toxic spraying

– Phytophtora resistant potato GMO • 35 genes, 10-12 years, durable • Classical breeding: 1 R gene, 45 years, cross with Andes potato lose qualities

– Transgenic papaya resistant to ringspot virus • Dennis Gonsalves (Hawaii) • Pathogen derived resistance,

– vaccinate with PRSV coat protein gene – started in 1991, demonstration to farmers 1997 – 1999 – present: Hawaii island Puna all papaya are transgenic

• Bad example – Roundup Ready

• Excessive spraying throughout cropping season • Residues in food

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Personal comments • Next generation should be to consumer benefit • Relative advantage must be obvious to consumer

– e.g. nutritional value (β-carotene, iron, folate, fatty acid composition) – health benefits (amylose) – sustainability – ornamental (flower and plant architecture) – pest and disease resistance

• Off-putting terms – Genetic, modified, engineered, TALENs, editing, Zinc fingers

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