Isolation of local bacterial capable of degrading halogenated compounds and analysis of putative haloacid permease gene

3-chloropropionic acid and 2,2-dichloropropionic acid are synthetic halogenated compounds used in herbicide. A bacterium isolated from a soil sample and characterised as Rhodococcus sp. by 16S rRNA analysis, was able to degrade and utilised 3-chloropropionate as the sole source of carbon and energy....

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Main Author: Ng, Hong Jing
Format: Thesis
Language:English
Published: 2007
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Online Access:http://eprints.utm.my/id/eprint/6798/1/NgHongJingMFS2007.pdf
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spelling my.utm.67982018-08-30T08:03:52Z http://eprints.utm.my/id/eprint/6798/ Isolation of local bacterial capable of degrading halogenated compounds and analysis of putative haloacid permease gene Ng, Hong Jing QH301 Biology 3-chloropropionic acid and 2,2-dichloropropionic acid are synthetic halogenated compounds used in herbicide. A bacterium isolated from a soil sample and characterised as Rhodococcus sp. by 16S rRNA analysis, was able to degrade and utilised 3-chloropropionate as the sole source of carbon and energy. This was supported by the ability of the bacterium to grow on 20 mM 3-chloropropionate with a doubling time of 11.72 hours. The utilisation of 3-chloropropionate was also confirmed by detection of 3-chloropropionate depletion in the medium using HPLC. Cell free extract of Rhodococcus sp. had an enzyme specific activity of 0.013 µmol Cl-/min/mg protein towards 3-chloropropionate. Another bacterium isolated from the same soil sample and identified as Methylobacterium sp. by 16S rRNA analysis was found to be able to degrade 2,2-dichloropropionate. The bacterium grew in 20mM 2,2-dichloropropionate minimal medium with a doubling time of 20.32 hours. Degradation of 2,2-dichloropropionate was further confirmed by detection of 2,2- dichloropropionate depletion in growth medium by HPLC. Cell free extract prepared from the cell showed 0.039 µmol Cl-/min/mg protein specific activity towards 2,2-dichloropropionate. A putative haloacid permease gene (dehrP) from Rhizobium sp. was subcloned into Novagen pET 43.1a plasmid. The newly constructed plasmid was designated as pHJ. The cloned gene was sequenced and analysed using various online analysis tools. DehrP has a calculated molecular weight of 45 kDa and an isoelectric point of 9.78. The nucleotide sequence of dehrP showed significant homology (86%) with the putative mono-chloropropionic acid permease from Agrobacterium sp. NHG3 and 62 % homology with the haloacid specific transferase from Burkholderia sp. 2007-02 Thesis NonPeerReviewed application/pdf en http://eprints.utm.my/id/eprint/6798/1/NgHongJingMFS2007.pdf Ng, Hong Jing (2007) Isolation of local bacterial capable of degrading halogenated compounds and analysis of putative haloacid permease gene. Masters thesis, Universiti Teknologi Malaysia, Faculty of Science. http://dms.library.utm.my:8080/vital/access/manager/Repository/vital:62525
institution Universiti Teknologi Malaysia
building UTM Library
collection Institutional Repository
continent Asia
country Malaysia
content_provider Universiti Teknologi Malaysia
content_source UTM Institutional Repository
url_provider http://eprints.utm.my/
language English
topic QH301 Biology
spellingShingle QH301 Biology
Ng, Hong Jing
Isolation of local bacterial capable of degrading halogenated compounds and analysis of putative haloacid permease gene
description 3-chloropropionic acid and 2,2-dichloropropionic acid are synthetic halogenated compounds used in herbicide. A bacterium isolated from a soil sample and characterised as Rhodococcus sp. by 16S rRNA analysis, was able to degrade and utilised 3-chloropropionate as the sole source of carbon and energy. This was supported by the ability of the bacterium to grow on 20 mM 3-chloropropionate with a doubling time of 11.72 hours. The utilisation of 3-chloropropionate was also confirmed by detection of 3-chloropropionate depletion in the medium using HPLC. Cell free extract of Rhodococcus sp. had an enzyme specific activity of 0.013 µmol Cl-/min/mg protein towards 3-chloropropionate. Another bacterium isolated from the same soil sample and identified as Methylobacterium sp. by 16S rRNA analysis was found to be able to degrade 2,2-dichloropropionate. The bacterium grew in 20mM 2,2-dichloropropionate minimal medium with a doubling time of 20.32 hours. Degradation of 2,2-dichloropropionate was further confirmed by detection of 2,2- dichloropropionate depletion in growth medium by HPLC. Cell free extract prepared from the cell showed 0.039 µmol Cl-/min/mg protein specific activity towards 2,2-dichloropropionate. A putative haloacid permease gene (dehrP) from Rhizobium sp. was subcloned into Novagen pET 43.1a plasmid. The newly constructed plasmid was designated as pHJ. The cloned gene was sequenced and analysed using various online analysis tools. DehrP has a calculated molecular weight of 45 kDa and an isoelectric point of 9.78. The nucleotide sequence of dehrP showed significant homology (86%) with the putative mono-chloropropionic acid permease from Agrobacterium sp. NHG3 and 62 % homology with the haloacid specific transferase from Burkholderia sp.
format Thesis
author Ng, Hong Jing
author_facet Ng, Hong Jing
author_sort Ng, Hong Jing
title Isolation of local bacterial capable of degrading halogenated compounds and analysis of putative haloacid permease gene
title_short Isolation of local bacterial capable of degrading halogenated compounds and analysis of putative haloacid permease gene
title_full Isolation of local bacterial capable of degrading halogenated compounds and analysis of putative haloacid permease gene
title_fullStr Isolation of local bacterial capable of degrading halogenated compounds and analysis of putative haloacid permease gene
title_full_unstemmed Isolation of local bacterial capable of degrading halogenated compounds and analysis of putative haloacid permease gene
title_sort isolation of local bacterial capable of degrading halogenated compounds and analysis of putative haloacid permease gene
publishDate 2007
url http://eprints.utm.my/id/eprint/6798/1/NgHongJingMFS2007.pdf
http://eprints.utm.my/id/eprint/6798/
http://dms.library.utm.my:8080/vital/access/manager/Repository/vital:62525
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score 13.209306