The Asian Journal of Horticulture

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Efficient and Simple Procedure for Isolation Ofrna from Pulp and Peel Tissues of Ripe Banana


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1 National Research Centre for Banana (ICAR), Trichy T.N., India
     

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Sensitive techniques of molecular biology, such as identification of differentially expressed genes, transcriptional profiling etc., require a high quality RNA in suitable quantities. Isolation of good quality RNA from banana pulp and peel tissues is troublesome and challenging owing to rich phenolic compounds and polysaccharides that coprecipitate with nucleic acids. Interaction of phenols with nucleic acids leads to oxidation and degradation of RNA making it unsuitable for downstream processes. We have developed a protocol to isolate good quality RNA from banana fruit pulp and peel tissues. This involves two precipitation steps with sodium acetate with 100 per cent ethanol and reducing the precipitation time which led to the reduction in loss of RNA and risk of degradation. The protocol developed is simple, fast and can extract 81.85 and 40.54 μg/g of pulp and peel tissues, respectively. The absorbance ranged from 1.9-2.0 at the ratio of 260/280 indicating very high quality of RNA suitable for molecular analyses. RNA purity was confirmed through reverse transcription-polymerase chain reaction (RT-PCR) by using-1,3 glucanase primer pair. The clear banding pattern obtained in RT-PCR analysis revealed that RNA isolated through this protocol could be used for further downstream processes.

Keywords

Banana, Ripe Fruit, Pulp, Peel, RNA Isolation
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  • Efficient and Simple Procedure for Isolation Ofrna from Pulp and Peel Tissues of Ripe Banana

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Authors

S. Backiyarani
National Research Centre for Banana (ICAR), Trichy T.N., India
S. Uma
National Research Centre for Banana (ICAR), Trichy T.N., India
M. S. Saraswathi
National Research Centre for Banana (ICAR), Trichy T.N., India
A. Saravankumar
National Research Centre for Banana (ICAR), Trichy T.N., India

Abstract


Sensitive techniques of molecular biology, such as identification of differentially expressed genes, transcriptional profiling etc., require a high quality RNA in suitable quantities. Isolation of good quality RNA from banana pulp and peel tissues is troublesome and challenging owing to rich phenolic compounds and polysaccharides that coprecipitate with nucleic acids. Interaction of phenols with nucleic acids leads to oxidation and degradation of RNA making it unsuitable for downstream processes. We have developed a protocol to isolate good quality RNA from banana fruit pulp and peel tissues. This involves two precipitation steps with sodium acetate with 100 per cent ethanol and reducing the precipitation time which led to the reduction in loss of RNA and risk of degradation. The protocol developed is simple, fast and can extract 81.85 and 40.54 μg/g of pulp and peel tissues, respectively. The absorbance ranged from 1.9-2.0 at the ratio of 260/280 indicating very high quality of RNA suitable for molecular analyses. RNA purity was confirmed through reverse transcription-polymerase chain reaction (RT-PCR) by using-1,3 glucanase primer pair. The clear banding pattern obtained in RT-PCR analysis revealed that RNA isolated through this protocol could be used for further downstream processes.

Keywords


Banana, Ripe Fruit, Pulp, Peel, RNA Isolation