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Research Detail

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Pronabananda  Das
Department of  Botany, University of   Dhaka,Dhaka-1000, Bangladesh.

Aneesa Ansari
Department of Botany, University of Dhaka,Dhaka-1000, Bangladesh.

Mohammad Nurul Islam
Department of Botany, University of Dhaka,Dhaka-1000, Bangladesh.

R. H. Sarker
Department of Botany, University of Dhaka,Dhaka-1000, Bangladesh

An  in   vitro   regeneration   and   Agrobacterium? mediated  genetic  transformation   protocol   was  optimized  for  a   local  tomato  variety,  BARI  Tomato? 8  using  cotyledonary   leaf   and   hypocotyls   explants.   The   explants   were  treated  with  various  growth  regulators   in   MS  at   different   concentrations   and   combinations.  Highest  number  of   multiple  shoot  induction  was  observed  from  both  the   explants   cultured   in   MS  supplemented  with  8.88  μ M  BAP   and   0.57  μ M  IAA.  Half   strength   of  MS  supplemented  with 1.14  μ M  IAA   was found   to   be  the   best   for  root   induction  from  excised  shoots.  Agrobacterium  mediated  genetic  transformation   was  carried  using  pBI121  plasmid  harboring β?glucuronidase  (GUS)   reporter   and   nptII  selectable  marker  genes.   Transient  GUS  assay  confirmed   that   both  the   explants   pre?cultured   for  two   days  showed   best   transformation   efficiency  in   bacterial   suspension   having  optical   density  (OD)  of   0.8  (at  600  nm)   for  15  min  and   co ? cultivation   period   of   3   days.  The   shoots  regenerated  from  transformed   cotyledonary   leaf   explants   survived   at   200  mg/l  kanamycin   selection.  The   presence   of   expected   amplicon  corresponding  to   the   GUS  gene  was  confirmed   by  PCR.  This   protocol   paves  a   way   for  developing   disease  resistant   tomato  variety  using  target  gene/s. 

  Genetic   transformation,  Agrobacterium,  BARI  Tomato
  Bangladesh Agricultural Research Institute, Joydebpur, Gazipur
  
  
  Variety and Species
  Tomato

To   establish   an  efficient   and   reproducible   regeneration   and   Agrobacterium mediated  genetic  transformation   protocol   for  a   farmer   popular  tomato  variety  in   Bangladesh  such  as;  BARI  Tomato8  variety  using  selectable  and  screenable   marker genes.

The   seeds  of   the   tomato  variety  BARI  Tomato? 8   were  collected   from  Bangladesh  Agricultural  Research   Institute   (BARI),  Joydebpur,   Gazipur.   To  generate   explants,   the   seeds  of   BARI  Tomato?8   were  treated  in   0.1%  (v/v)  mercuric   chloride   for  10 ? 15   min  with  vigorous   shaking,   washed  three  times   with  autoclaved   distilled   water  and   inoculated   onto   the   cotton   bed   for  germination.   These  seeds  were  kept   in   the   dark  till  the   germination  took   place  and   finally   transferred   to   16? hourslight  and   8   hours  dark  condition  at   25  ±   2 º C  in   growth  room.   The   seedlings  were  used  for  explants   preparation.  The   cotyledonary   leaf   and   hypocotyls   were  first   separated.   The   leaves   were  cut  at   tip  and   the   base, removing  the   meristematic  tissue,   whereas  the   hypocotyls   were  segmented   into   approximately  0.5  cm  in   size.  MS  in   combination   with  different   hormones  were  used  for  regeneration   and   transformation   experiments.   The   pH  of   the   medium  was  adjusted   to   5.8.   The   medium  was  then   autoclaved.  Different   combinations   of   hormone  andsupplements   like   IAA,  Kn,  GA3 ,   NAA,  BAP   and   2,4?D  were  added   for  multiple  shoot  regeneration. In   case   of   rooting,   three  types   of   media  were  used,  i.e.  MS  containing   1.14  μ M  IAA,  half   strength   of  MS  containing   0.98  μ M  IBA   and   half   strength   of   MS  containing   1.14  μ M  IAA.  The   antibiotic  kanamycin   was  used  to   select   the   transformed   plants   after  infection   with  Agrobacterium  tumefaciens   carrying   pBI121  plasmid  containing   nptII  gene. Agrobacterium  tumefaciens   strain   LBA4404   containing   plasmid  pBI121  of   14  kb  (binary  vector)  was  used  for  the   transformation.   This   binary   vector   contains   uidA  gene encoding  GUS,  driven   by  CaMV   35S   promoter  and   NOS  terminator   and    nptII  gene  encoding  neomycin  phosphotransferase   II   conferring   kanamycin   resistance  within   the   right  border   (RB)   and   left   border   (LB)   region   of   the   T? DNA.  The   bacterium  also   contains   plasmid  pAL4404   which  is   a   disarmed  Ti   plasmid  (132   kb)  containing   the   virulence genes.  Histochemical  assay  was  performed   to   visualize   GUS  activity.   The   leaf   tissues   which  survived   the   highest  kanamycin   concentration  was  selected   and   incubated   in   GUS  histochemical  buffer   [50  mM  sodium  phosphate,   pH7.0;   50   mM  EDTA,  pH  8.0;  0.5  mM  K3Fe(CN)6;  0.5  mMK4Fe(CN)6;   0.1%  triton   X? 100;   1.0  mM  X? gluc   (5 ? bromo ? 4? chloro ?3 ?indolyl  β ? D?glucuronide)]  at   37°C  for  up  to   24  hrs.   Chlorophyll  in  leaf   tissues   was  subsequently   removed   by  washing  with  70%   alcohol  after  every  3  days.  For  molecular  analysis,   the   genomic   DNA  was  isolated   from  the   plantlets   which  survived   under   the   highest  selection   pressure  using  modified  CTAB  method. Using  the   isolated   DNA,  PCR   was  performed   with  GUSA ? 769  (nucleotide   sequence:  TGG  CTG  TGA  ACG  CAC  AGT  TCA)  and   GUSA ? 10   (nucleotide   sequence:  CCT  GTA  GAA  ACC  CCA  ACC  CG)   primers  for  molecular  confirmation   of   the   genetic  transformation.   The   conditions   for  PCR   was  95°C  for  5   min,  94°C  for  1   min,   56°C  for  1   min,  72°C  for  1   min  and   repeated   for  30   cycles.   The   final   extension  was  maintained  72°C  for  10   minutes and  paused at   4°C.   The  amplified  band  was checked  in   the   agarose gel.  

 

  Plant  Tissue   Cult.  &  Biotech. 25(1):   87-97,  2015   (June)
  
Funding Source:
  

The   regeneration   response   of   the   cotelydonary   leaf   explants   was  better  than   hypocotyls   and   subsequently,  transgenic   plants   obtained   from  cotyledonary   leaf   explants   following  the   regeneration   protocol.   Therefore,  this   protocol   endeavors   a  new   and   efficient   way   for  obtaining transgenic   plants   which  can   be  used  to   transfer   useful   candidate  genes  conferring   disease, insect   and   pest   resistance  in   the  BARI  Tomato? 8  variety  of  Bangladesh. 

  Journal
  


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