An efficient protocol for isolation of functional RNA from peel tissue of different banana (Musa spp.) cultivars for gene expression studies on anthracnose development

<p>Extraction of good quality RNA in larger quantities is a prerequisite for gene expression studies. Existing protocols for RNA extraction from banana pulp tissues were not successful on peel tissues of banana (Musa spp) as they contain higher concentrations of polyphenols, polysaccharides an...

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Main Authors: U. M. Aruna Kumara, Devika M. De Costa
Format: Article
Language:English
Published: Postgraduate Institute of Agriculture, University of Peradeniya 2015-11-01
Series:Tropical Agricultural Research
Subjects:
Online Access:https://tar.sljol.info/articles/8096
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spelling doaj-a2e28e1d228840b8afd869e6603477032020-11-25T01:52:35ZengPostgraduate Institute of Agriculture, University of PeradeniyaTropical Agricultural Research1016-14222015-11-0126210.4038/tar.v26i2.80966022An efficient protocol for isolation of functional RNA from peel tissue of different banana (Musa spp.) cultivars for gene expression studies on anthracnose developmentU. M. Aruna Kumara0Devika M. De Costa1University of PeradeniyaUniversity of Peradeniya<p>Extraction of good quality RNA in larger quantities is a prerequisite for gene expression studies. Existing protocols for RNA extraction from banana pulp tissues were not successful on peel tissues of banana (Musa spp) as they contain higher concentrations of polyphenols, polysaccharides and latex. This study developed a new protocol by modifying the existing protocols. The modifications included combining of pre-warmed Tris-Borate extraction buffer, incorporation of CTAB in the extraction buffer, incubation in extraction buffer at 65<sup>o</sup>C for one hour, and a three-day long extraction procedure with phenol, phenol:chloroform (1:1) and chloroform:isoamyl alcohol (24:1) together with centrifugation steps at high speeds (i.e. 12,000 –14,000 rpm). Spectrophotometric analysis of the extracted RNA, denaturing agarose gel electrophoresis, cDNA library construction, sequence information of cDNA inserts and RT-PCR confirmed the quality of RNA extracted by the method developed in the present study for gene expression work. Furthermore, it is shown that the developed method is useful to extract good quality RNA from peel tissues of a range of dessert- and cooking-type banana cultivars.</p><p>Tropical Agricultural Research Vol. 26 (2): 329 – 342 (2015)</p>https://tar.sljol.info/articles/8096cdna library construction, colletotricummusae, rna extraction, rt-pcr
collection DOAJ
language English
format Article
sources DOAJ
author U. M. Aruna Kumara
Devika M. De Costa
spellingShingle U. M. Aruna Kumara
Devika M. De Costa
An efficient protocol for isolation of functional RNA from peel tissue of different banana (Musa spp.) cultivars for gene expression studies on anthracnose development
Tropical Agricultural Research
cdna library construction, colletotricummusae, rna extraction, rt-pcr
author_facet U. M. Aruna Kumara
Devika M. De Costa
author_sort U. M. Aruna Kumara
title An efficient protocol for isolation of functional RNA from peel tissue of different banana (Musa spp.) cultivars for gene expression studies on anthracnose development
title_short An efficient protocol for isolation of functional RNA from peel tissue of different banana (Musa spp.) cultivars for gene expression studies on anthracnose development
title_full An efficient protocol for isolation of functional RNA from peel tissue of different banana (Musa spp.) cultivars for gene expression studies on anthracnose development
title_fullStr An efficient protocol for isolation of functional RNA from peel tissue of different banana (Musa spp.) cultivars for gene expression studies on anthracnose development
title_full_unstemmed An efficient protocol for isolation of functional RNA from peel tissue of different banana (Musa spp.) cultivars for gene expression studies on anthracnose development
title_sort efficient protocol for isolation of functional rna from peel tissue of different banana (musa spp.) cultivars for gene expression studies on anthracnose development
publisher Postgraduate Institute of Agriculture, University of Peradeniya
series Tropical Agricultural Research
issn 1016-1422
publishDate 2015-11-01
description <p>Extraction of good quality RNA in larger quantities is a prerequisite for gene expression studies. Existing protocols for RNA extraction from banana pulp tissues were not successful on peel tissues of banana (Musa spp) as they contain higher concentrations of polyphenols, polysaccharides and latex. This study developed a new protocol by modifying the existing protocols. The modifications included combining of pre-warmed Tris-Borate extraction buffer, incorporation of CTAB in the extraction buffer, incubation in extraction buffer at 65<sup>o</sup>C for one hour, and a three-day long extraction procedure with phenol, phenol:chloroform (1:1) and chloroform:isoamyl alcohol (24:1) together with centrifugation steps at high speeds (i.e. 12,000 –14,000 rpm). Spectrophotometric analysis of the extracted RNA, denaturing agarose gel electrophoresis, cDNA library construction, sequence information of cDNA inserts and RT-PCR confirmed the quality of RNA extracted by the method developed in the present study for gene expression work. Furthermore, it is shown that the developed method is useful to extract good quality RNA from peel tissues of a range of dessert- and cooking-type banana cultivars.</p><p>Tropical Agricultural Research Vol. 26 (2): 329 – 342 (2015)</p>
topic cdna library construction, colletotricummusae, rna extraction, rt-pcr
url https://tar.sljol.info/articles/8096
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