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High frequency adventitious root and
   shoot regeneration in recalcitrant
         sweet potato cultivars




                        Abel Sefasi
             Department of Agricultural Production
                    Makerere University

Supervisors:
Dr. G. Ssemakula                        Regional RUFORUM
Dr. A. Kiggundu                         Biennial Conference,
Dr. M. Ghislain                         24-28 Sept. 2012,
Dr. S. Mukasa                           Entebbe Uganda
Background
 Sweetpotato is seventh among the food crops in
  annual production in the world (FAO, 2007)

 Uganda is the biggest producer in Africa at 1.8
  million tons (FAO, 2010)

 Weevils, Cylas puncticollis and C. brunneus cause
  production losses over 28% (Kiiza et al., 2009)

 Heritability of the resistance trait is extremely low
  and not well understood (Stevenson et al., 2009)

 Three Bt Cry proteins (Cry7Aa1, Cry3Ca1, ET33-
  34) active against the two African weevil species
  identified (Ekobu et al 2010)
Justification
 The genes expressing the Cry proteins have been
  assembled into a plasmid gene construct

 Agrobacterium-mediated genetic transformation is the
  option

 However production of transgenic sweetpotato requires
  an in vitro protocol for regeneration                                        nos promoter
                                                                                    nptII                 gSPOA1 promoter
                                                                      3' 35S
                                                                 LB
                                             kanamycin (R)                                                                       cry3Ca1
 Sweetpotato is considered                 pBR322 ori                                                                                     3' gSPOA1

  recalcitrant to both          pBR322 bom site
                                                                                              pCIP84

  transformation and in vitro
                                                                                              14602 bp
                                                                                                                                           ß-amy promoter
                                                  pVS1-REP

  regeneration
                                                                                                                            cry7Aa1
                                                             pVS1 Stab
                                                                                                              3' ß-amy
                                                                                                         RB
Justification
 It is necessary that there are very few ‘escapes’ and no
  chimeric plants resulting from regeneration

 Two protocols that have been reported for regeneration of
  some cultivars of sweetpotato
                                                                                                                   b

                                                          a

                  Meristems
                  excision      Embryogenic calli              4–5          Transformation 1
 4 – 5 weeks      (6 weeks in                                  weeks        day in MIB medium
                                transformation (2
                  dark)         days in dark)                               in dark, then 4 days
                                                                            to medium with 2,4-
                                                                            D
    High transformation frequency
                                           medium with 2,5-T
                                           (2 months)
                                                                       Short
                                                                       duration
                                                                                                   Medium with Kin or
                                                                                                   Zea subculture
                                                                                                   each 15 days per 2
                                                                                  Regenerants to   months
                       Medium with         Medium with ABA
 Regenerants to                                                                   MPB medium
                       GA3 (2 months)      (3 months)
 MPB medium
Objectives
Main objective:
 The main objective of this study is to genetically transform
  selected Ugandan sweetpotato cultivars with weevil resistance
  genes

Specific objectives:
 To develop a tissue culture protocol for regeneration of selected
  Ugandan sweetpotato cultivars

 To develop a protocol for genetic transformation of Ugandan
  sweetpotato cultivars to improve weevil resistance

 To study expression patterns of transgenes and their efficacy
  against Ugandan sweetpotato weevils after genetic
Materials and methods
 Media: MS, myo-inositol (0.1 g l-1), sucrose
  (30 g l-1) and 1 ml l-1 sweetpotato vitamin
  stock, pH 5.8

 Cultivars: Kyebandula and Bwanjule

 Explant types: whole leaves and stem
  internode

 Growth regulators: TDZ (0.5, 2.0, 4.0 µM)
  and TDZ with NAA (0.25 µM)

 Completely Randomised Design
Data collection and management

 Three replicates with 30 explants per rep

 Each rep had 3 petri dishes each containing 10 explants

 Data on number of shoots regenerated was collected 12
  weeks after culture initiation

 Statistical analyses done using ANOVA

 Means were compared using the LSD test at the P ≤ 0.05
  level
Results
 Shoot regeneration was successfully achieved

 Regeneration through adventitious shoots / organogenesis

 Cultivar type, [TDZ], explant type significantly (P ≤ 0.05)
  affected the no. of adventious buds formed per explants
  (not presented).

 Both type of cultivar and concentration of TDZ did not affect
  shoot regeneration efficiency

 Stem explants gave a significantly (p < 0.05) high
  regeneration efficiency for all TDZ concentrations
Results cont’d




Effect of TDZ concentration (0.5, 2.0, 4.0 µM) on shoot
regeneration frequency from stem and leaf explants of
Bwanjule and Kyebandula cultivars
F-Test: Effect of TDZ concentration (µM), types of
  explants of cultivar on bud induction and shoot
               regeneration frequency

                               Explants forming Shoots per
                               shoots (Frequency) explant
                                                  (No.)
Cultivar                       0.134           0.342
Explant                        0.312           <.001
TDZ concentration (µM)         0.168           0.344
Cultivar X Explant             0.498           1
Cultivar X TDZ concentration   0.193           0.477
Explant X TDZ concentration    0.512           0.943
Results cont’d




Effect of TDZ concentration (0.5, 2.0, 4.0 µM) in the
presence of NAA (0.25 µM) on shoot regeneration
frequency from stem and leaf explants of Bwanjule
and Kyebandula cultivars
(a) Adventitious bud
Results cont’d
                     protrusion along the
                     length of petiole of leaf
                     explants after 2 weeks
                 (b) Elongation of
                     adventitious buds
                     leading to development
                     of shoots
                 (c) Development of multiple
                     adventitious shoots on
                     stem internode explants
                 (d) Growth of plants in soil
                     4 weeks after
                     acclimatisation in the
                     greenhouse.
Discussion
 We have regenerated cultivars that were recalcitrant to
  common protocols used in in vitro regeneration

 The results achieved in this study are very important for
  the breeding of I. batatas, particularly African cultivars,
  which have been reported to be difficult to regenerate in
  vitro.

 Only two cultivars were tested. It is interesting that cultivar
  type did not show significant effect on regeneration
  efficiency

 These results confirm that sweetpotato regeneration in
  vitro is cultivar-dependent
Conclusions
• A reliable adventitious regeneration protocol has been
  established for I. batatas cultivars which have not been
  regenerated before

• This protocol has potential to be extended to the
  regeneration of other economically important I. batatas
  cultivars

• The ultimate goal is to apply this protocol in genetic
  transformation for improvement of I. batatas traits,
  especially for resistance to weevils.

• Most I. batatas cultivars that were thought to be recalcitrant
  can be regenerated following optimisation of media
  composition.
Recommendations

 Most adventitious buds failed to turn into shoots

 It is recommended that culture systems be developed for
  efficient adventitious regeneration to be effectively induced
  in a wide range of cultivars
Progress with papers and manuscript
Papers submitted to peer reviewed journals:
1. Induction of somatic embryogenesis in recalcitrant sweetpotato
   (Ipomoea batatas L.) varieties. Afr. Journ. Biotech. Responded to
   reviewers comments’ in Aug. 2012

2. Thidiazuron-induced efficient adventitious bud and shoot
   regeneration in recalcitrant sweetpotato. Afr. Crop Sci. Journ.
   Submitted Aug. 2012

Papers in early draft form:
1. Genetic transformation of recalcitrant sweetpotato through somatic
   embryogenesis from stem internodes. In vitro cell Dev. Biol. Plant.

2. 2,4-dichlorophenoxyacetic acid confirms recalcitrance to somatic
   embryogenesis in some important African sweetpotato cultivars.
   Short communication. Plant Phys
Thank you

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High frequency adventitious root and shoot regeneration in recalcitrant sweet potato cultivars

  • 1. High frequency adventitious root and shoot regeneration in recalcitrant sweet potato cultivars Abel Sefasi Department of Agricultural Production Makerere University Supervisors: Dr. G. Ssemakula Regional RUFORUM Dr. A. Kiggundu Biennial Conference, Dr. M. Ghislain 24-28 Sept. 2012, Dr. S. Mukasa Entebbe Uganda
  • 2. Background  Sweetpotato is seventh among the food crops in annual production in the world (FAO, 2007)  Uganda is the biggest producer in Africa at 1.8 million tons (FAO, 2010)  Weevils, Cylas puncticollis and C. brunneus cause production losses over 28% (Kiiza et al., 2009)  Heritability of the resistance trait is extremely low and not well understood (Stevenson et al., 2009)  Three Bt Cry proteins (Cry7Aa1, Cry3Ca1, ET33- 34) active against the two African weevil species identified (Ekobu et al 2010)
  • 3. Justification  The genes expressing the Cry proteins have been assembled into a plasmid gene construct  Agrobacterium-mediated genetic transformation is the option  However production of transgenic sweetpotato requires an in vitro protocol for regeneration nos promoter nptII gSPOA1 promoter 3' 35S LB kanamycin (R) cry3Ca1  Sweetpotato is considered pBR322 ori 3' gSPOA1 recalcitrant to both pBR322 bom site pCIP84 transformation and in vitro 14602 bp ß-amy promoter pVS1-REP regeneration cry7Aa1 pVS1 Stab 3' ß-amy RB
  • 4. Justification  It is necessary that there are very few ‘escapes’ and no chimeric plants resulting from regeneration  Two protocols that have been reported for regeneration of some cultivars of sweetpotato b a Meristems excision Embryogenic calli 4–5 Transformation 1 4 – 5 weeks (6 weeks in weeks day in MIB medium transformation (2 dark) days in dark) in dark, then 4 days to medium with 2,4- D High transformation frequency medium with 2,5-T (2 months) Short duration Medium with Kin or Zea subculture each 15 days per 2 Regenerants to months Medium with Medium with ABA Regenerants to MPB medium GA3 (2 months) (3 months) MPB medium
  • 5. Objectives Main objective:  The main objective of this study is to genetically transform selected Ugandan sweetpotato cultivars with weevil resistance genes Specific objectives:  To develop a tissue culture protocol for regeneration of selected Ugandan sweetpotato cultivars  To develop a protocol for genetic transformation of Ugandan sweetpotato cultivars to improve weevil resistance  To study expression patterns of transgenes and their efficacy against Ugandan sweetpotato weevils after genetic
  • 6. Materials and methods  Media: MS, myo-inositol (0.1 g l-1), sucrose (30 g l-1) and 1 ml l-1 sweetpotato vitamin stock, pH 5.8  Cultivars: Kyebandula and Bwanjule  Explant types: whole leaves and stem internode  Growth regulators: TDZ (0.5, 2.0, 4.0 µM) and TDZ with NAA (0.25 µM)  Completely Randomised Design
  • 7. Data collection and management  Three replicates with 30 explants per rep  Each rep had 3 petri dishes each containing 10 explants  Data on number of shoots regenerated was collected 12 weeks after culture initiation  Statistical analyses done using ANOVA  Means were compared using the LSD test at the P ≤ 0.05 level
  • 8. Results  Shoot regeneration was successfully achieved  Regeneration through adventitious shoots / organogenesis  Cultivar type, [TDZ], explant type significantly (P ≤ 0.05) affected the no. of adventious buds formed per explants (not presented).  Both type of cultivar and concentration of TDZ did not affect shoot regeneration efficiency  Stem explants gave a significantly (p < 0.05) high regeneration efficiency for all TDZ concentrations
  • 9. Results cont’d Effect of TDZ concentration (0.5, 2.0, 4.0 µM) on shoot regeneration frequency from stem and leaf explants of Bwanjule and Kyebandula cultivars
  • 10. F-Test: Effect of TDZ concentration (µM), types of explants of cultivar on bud induction and shoot regeneration frequency Explants forming Shoots per shoots (Frequency) explant (No.) Cultivar 0.134 0.342 Explant 0.312 <.001 TDZ concentration (µM) 0.168 0.344 Cultivar X Explant 0.498 1 Cultivar X TDZ concentration 0.193 0.477 Explant X TDZ concentration 0.512 0.943
  • 11. Results cont’d Effect of TDZ concentration (0.5, 2.0, 4.0 µM) in the presence of NAA (0.25 µM) on shoot regeneration frequency from stem and leaf explants of Bwanjule and Kyebandula cultivars
  • 12. (a) Adventitious bud Results cont’d protrusion along the length of petiole of leaf explants after 2 weeks (b) Elongation of adventitious buds leading to development of shoots (c) Development of multiple adventitious shoots on stem internode explants (d) Growth of plants in soil 4 weeks after acclimatisation in the greenhouse.
  • 13. Discussion  We have regenerated cultivars that were recalcitrant to common protocols used in in vitro regeneration  The results achieved in this study are very important for the breeding of I. batatas, particularly African cultivars, which have been reported to be difficult to regenerate in vitro.  Only two cultivars were tested. It is interesting that cultivar type did not show significant effect on regeneration efficiency  These results confirm that sweetpotato regeneration in vitro is cultivar-dependent
  • 14. Conclusions • A reliable adventitious regeneration protocol has been established for I. batatas cultivars which have not been regenerated before • This protocol has potential to be extended to the regeneration of other economically important I. batatas cultivars • The ultimate goal is to apply this protocol in genetic transformation for improvement of I. batatas traits, especially for resistance to weevils. • Most I. batatas cultivars that were thought to be recalcitrant can be regenerated following optimisation of media composition.
  • 15. Recommendations  Most adventitious buds failed to turn into shoots  It is recommended that culture systems be developed for efficient adventitious regeneration to be effectively induced in a wide range of cultivars
  • 16. Progress with papers and manuscript Papers submitted to peer reviewed journals: 1. Induction of somatic embryogenesis in recalcitrant sweetpotato (Ipomoea batatas L.) varieties. Afr. Journ. Biotech. Responded to reviewers comments’ in Aug. 2012 2. Thidiazuron-induced efficient adventitious bud and shoot regeneration in recalcitrant sweetpotato. Afr. Crop Sci. Journ. Submitted Aug. 2012 Papers in early draft form: 1. Genetic transformation of recalcitrant sweetpotato through somatic embryogenesis from stem internodes. In vitro cell Dev. Biol. Plant. 2. 2,4-dichlorophenoxyacetic acid confirms recalcitrance to somatic embryogenesis in some important African sweetpotato cultivars. Short communication. Plant Phys