CLC number: Q503
On-line Access: 2024-08-27
Received: 2023-10-17
Revision Accepted: 2024-05-08
Crosschecked: 2012-02-29
Cited: 14
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Muhammad Abubakkar Azmat, Iqrar Ahmad Khan, Hafiza Masooma Naseer Cheema, Ishtiaq Ahmad Rajwana, Ahmad Sattar Khan, Asif Ali Khan. Extraction of DNA suitable for PCR applications from mature leaves of Mangifera indica L.[J]. Journal of Zhejiang University Science B, 2012, 13(4): 239-243.
@article{title="Extraction of DNA suitable for PCR applications from mature leaves of Mangifera indica L.",
author="Muhammad Abubakkar Azmat, Iqrar Ahmad Khan, Hafiza Masooma Naseer Cheema, Ishtiaq Ahmad Rajwana, Ahmad Sattar Khan, Asif Ali Khan",
journal="Journal of Zhejiang University Science B",
volume="13",
number="4",
pages="239-243",
year="2012",
publisher="Zhejiang University Press & Springer",
doi="10.1631/jzus.B1100194"
}
%0 Journal Article
%T Extraction of DNA suitable for PCR applications from mature leaves of Mangifera indica L.
%A Muhammad Abubakkar Azmat
%A Iqrar Ahmad Khan
%A Hafiza Masooma Naseer Cheema
%A Ishtiaq Ahmad Rajwana
%A Ahmad Sattar Khan
%A Asif Ali Khan
%J Journal of Zhejiang University SCIENCE B
%V 13
%N 4
%P 239-243
%@ 1673-1581
%D 2012
%I Zhejiang University Press & Springer
%DOI 10.1631/jzus.B1100194
TY - JOUR
T1 - Extraction of DNA suitable for PCR applications from mature leaves of Mangifera indica L.
A1 - Muhammad Abubakkar Azmat
A1 - Iqrar Ahmad Khan
A1 - Hafiza Masooma Naseer Cheema
A1 - Ishtiaq Ahmad Rajwana
A1 - Ahmad Sattar Khan
A1 - Asif Ali Khan
J0 - Journal of Zhejiang University Science B
VL - 13
IS - 4
SP - 239
EP - 243
%@ 1673-1581
Y1 - 2012
PB - Zhejiang University Press & Springer
ER -
DOI - 10.1631/jzus.B1100194
Abstract: Good quality deoxyribonucleic acid (DNA) is the pre-requisite for its downstream applications. The presence of high concentrations of polysaccharides, polyphenols, proteins, and other secondary metabolites in mango leaves poses problem in getting good quality DNA fit for polymerase chain reaction (PCR) applications. The problem is exacerbated when DNA is extracted from mature mango leaves. A reliable and modified protocol based on the cetyltrimethylammonium bromide (CTAB) method for DNA extraction from mature mango leaves is described here. High concentrations of inert salt were used to remove polysaccharides; Polyvinylpyrrolidone (PVP) and β-mercaptoethanol were employed to manage phenolic compounds. Extended chloroform-isoamyl alcohol treatment followed by RNase treatment yielded 950‒1050 µg of good quality DNA, free of protein and RNA. The problems of DNA degradation, contamination, and low yield due to irreversible binding of phenolic compounds and coprecipitation of polysaccharides with DNA were avoided by this method. The DNA isolated by the modified method showed good PCR amplification using simple sequence repeat (SSR) primers. This modified protocol can also be used to extract DNA from other woody plants having similar problems.
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Open peer comments: Debate/Discuss/Question/Opinion
<1>
Mudassir Iqbal@AARI<asuaf@gmail.com>
2012-01-25 18:10:05
This is an excellent protocol i tried this protocol to extract DNA from mature leaves of mulberry. The DNA obtained was of very good quality.