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Author Biographies
J Kakuturu
Central Pennsylvania Laboratory for Biofuels, Penn State Harrisburg, 777 West Harrisburg Pike, Middletown, PA 17057, United States
PC Josekutty
Central Pennsylvania Laboratory for Biofuels, Penn State Harrisburg, 777 West Harrisburg Pike, Middletown, PA 17057, United States
S Potlakayala
Central Pennsylvania Laboratory for Biofuels, Penn State Harrisburg, 777 West Harrisburg Pike, Middletown, PA 17057, United States
M Reitzel
Central Pennsylvania Laboratory for Biofuels, Penn State Harrisburg, 777 West Harrisburg Pike, Middletown, PA 17057, United States
K Salim
Central Pennsylvania Laboratory for Biofuels, Penn State Harrisburg, 777 West Harrisburg Pike, Middletown, PA 17057, United States
S Charyulu
Central Pennsylvania Laboratory for Biofuels, Penn State Harrisburg, 777 West Harrisburg Pike, Middletown, PA 17057, United States
R Adeyiga
Cheyney University of Pennsylvania, 1837 University Circle, PO Box 200, Cheyney, PA 19319, United States
S Menon
Central Pennsylvania Laboratory for Biofuels, Penn State Harrisburg, 777 West Harrisburg Pike, Middletown, PA 17057, United States
SL Goldman
University of Toledo, 2801 Bancroft Street, Toledo, OH 43606, United States
P Patel
Central Pennsylvania Laboratory for Biofuels, Penn State Harrisburg, 777 West Harrisburg Pike, Middletown, PA 17057, United States
MJ Chorney
Central Pennsylvania Laboratory for Biofuels, Penn State Harrisburg, 777 West Harrisburg Pike, Middletown, PA 17057, United States
S Rudrabhatla
Central Pennsylvania Laboratory for Biofuels, Penn State Harrisburg, 777 West Harrisburg Pike, Middletown, PA 17057, United States
Main Article Content
Callus induction and RAPD analysis of Simarouba glauca DC
J Kakuturu
PC Josekutty
S Potlakayala
M Reitzel
K Salim
S Charyulu
R Adeyiga
S Menon
SL Goldman
P Patel
MJ Chorney
S Rudrabhatla
Abstract
Callus induction for somatic embryogenesis from Simarouba glauca DC leaf explants of three genotypes (S. glauca 5, S. glauca 19 and S. glauca 21) was studied. Leaf explants (leaf segments from basal, middle and tip of the leaves) were cultured on two types of nutrient media; SGC1 and SGC2. Both media contained Murashige and Skoog (MS) medium with vitamins: 100 mg/L ascorbic acid, 0.5 mg/L 6-benzylaminopurine (BAP), 0.5 to 5.0 mg/L NAA (1-napthaleneacetic acid), and 3.0 g/L sucrose. The SGC2 media additionally contained 0.5 to 5.0 mg/L 2,4-dichlorophenoxyacetic acid (2,4-D). SGC2 media generated better callusing response compared to SGC1, thus displaying the importance of using 2,4-D in combination with NAA for callus induction. MS medium containing 2.5 mg/L NAA (SGC1.5) was noted to be the most effective in the initiation of friable embryogenic callus. On the other hand, MS medium containing a combination of 2.0 mg/L NAA and 2.0 mg/L 2,4-D was effective in the early initiation of friable embryogenic callus. In addition, a higher frequency of callus formation was observed from basal leaf segment as compared to that from middle and apical leaf segments. A random amplified polymorphic DNA (RAPD) analysis was also performed to see the genetic differences between the three S. glauca genotypes used in this study. The performance of S. glauca 5 and S. glauca 19 for higher callus frequency over the S. glauca 21 could be attributed to the genotypic differences between these genotypes. Overall, our protocol using SGC 2.4 media yielded optimal results and is suitable for large scale micropropagation of S. glauca.
African Journal of Biotechnology, Vol 13(53) 4766-4774
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