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Isolation and Characterisation of Microbial DNA from Rain Tree Barks

Most microorganisms present in nature are uncultivable by standard techniques and functions of commensal bacteria remained largely uncovered. Metagenomics assessment to study microbial community on tree barks was not attempted from literature search. In this research, a metagenomics DNA extraction p...

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Main Author: Mun, Chee Onn
Format: Thesis
Language:English
Published: 2017
Subjects:
QR Microbiology
Online Access:http://eprints.intimal.edu.my/949/1/125.pdf
http://eprints.intimal.edu.my/949/
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spelling my-inti-eprints.9492017-11-14T08:22:08Z http://eprints.intimal.edu.my/949/ Isolation and Characterisation of Microbial DNA from Rain Tree Barks Mun, Chee Onn QR Microbiology Most microorganisms present in nature are uncultivable by standard techniques and functions of commensal bacteria remained largely uncovered. Metagenomics assessment to study microbial community on tree barks was not attempted from literature search. In this research, a metagenomics DNA extraction protocol by combining a series of lysis, extraction and purification methods was developed for high quality genomic DNA extraction of cultivable and uncultivable microorganisms present on local rain tree bark. Sodium dodecyle sulphate (SDS)-based extraction method with cetyltrimethyl ammonium bromide (CTAB) as strong DNA extraction buffer was carried out to extract metagenomes from two bark samples, namely orchid-colonised and non-orchid-colonised bark samples, followed by its qualitative (agarose gel electrophoresis) and quantitative (spectrophotometry) assessments. The quality of metagenomics DNA extracted was insufficient where the A260/A280 ratio was in range from 1.47 to 1.81, and low A260/A230 ratio obtained indicated the probability of contamination by humic substances and phenols. The metagenomic DNA was not suitable for cloning due to inability to be restriction digested by HindIII. The metagenomic DNA was accessed for 16S ribosomal RNA (rRNA) polymerase chain reaction (PCR) amplification and the results suggested that the purity of the metagenomics DNA was sufficient for PCR. Amplification results also indicated the presence of bacteria and fungi in high amount on the bark surface. The presence of archaea cannot be indicated due to unspecific amplification and no single band with the expected size was obtained. No difference between non-orchid and orchid-colonised bark samples in terms of amplified rDNA in the range of 8.2 to 14.1 ug, which were sufficient for next generation sequencing (NGS) for rain tree bark metagenomics study, specifically on the ecology of microorganisms on rain tree bark. 2017 Thesis NonPeerReviewed text en http://eprints.intimal.edu.my/949/1/125.pdf Mun, Chee Onn (2017) Isolation and Characterisation of Microbial DNA from Rain Tree Barks. Other thesis, INTI International University.
institution INTI International University
building INTI Library
collection Institutional Repository
continent Asia
country Malaysia
content_provider INTI International University
content_source INTI Institutional Repository
url_provider http://eprints.intimal.edu.my
language English
topic QR Microbiology
spellingShingle QR Microbiology
Mun, Chee Onn
Isolation and Characterisation of Microbial DNA from Rain Tree Barks
description Most microorganisms present in nature are uncultivable by standard techniques and functions of commensal bacteria remained largely uncovered. Metagenomics assessment to study microbial community on tree barks was not attempted from literature search. In this research, a metagenomics DNA extraction protocol by combining a series of lysis, extraction and purification methods was developed for high quality genomic DNA extraction of cultivable and uncultivable microorganisms present on local rain tree bark. Sodium dodecyle sulphate (SDS)-based extraction method with cetyltrimethyl ammonium bromide (CTAB) as strong DNA extraction buffer was carried out to extract metagenomes from two bark samples, namely orchid-colonised and non-orchid-colonised bark samples, followed by its qualitative (agarose gel electrophoresis) and quantitative (spectrophotometry) assessments. The quality of metagenomics DNA extracted was insufficient where the A260/A280 ratio was in range from 1.47 to 1.81, and low A260/A230 ratio obtained indicated the probability of contamination by humic substances and phenols. The metagenomic DNA was not suitable for cloning due to inability to be restriction digested by HindIII. The metagenomic DNA was accessed for 16S ribosomal RNA (rRNA) polymerase chain reaction (PCR) amplification and the results suggested that the purity of the metagenomics DNA was sufficient for PCR. Amplification results also indicated the presence of bacteria and fungi in high amount on the bark surface. The presence of archaea cannot be indicated due to unspecific amplification and no single band with the expected size was obtained. No difference between non-orchid and orchid-colonised bark samples in terms of amplified rDNA in the range of 8.2 to 14.1 ug, which were sufficient for next generation sequencing (NGS) for rain tree bark metagenomics study, specifically on the ecology of microorganisms on rain tree bark.
format Thesis
author Mun, Chee Onn
author_facet Mun, Chee Onn
author_sort Mun, Chee Onn
title Isolation and Characterisation of Microbial DNA from Rain Tree Barks
title_short Isolation and Characterisation of Microbial DNA from Rain Tree Barks
title_full Isolation and Characterisation of Microbial DNA from Rain Tree Barks
title_fullStr Isolation and Characterisation of Microbial DNA from Rain Tree Barks
title_full_unstemmed Isolation and Characterisation of Microbial DNA from Rain Tree Barks
title_sort isolation and characterisation of microbial dna from rain tree barks
publishDate 2017
url http://eprints.intimal.edu.my/949/1/125.pdf
http://eprints.intimal.edu.my/949/
_version_ 1644541348279222272
score 13.201949

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