KONSTRUKSI DAN EKSPRESI GEN DNA POLIMERASE MUTAN DELESI BAKTERI TERMOFILIK ISOLAT CIMANGGU DI Escherichia coli

KONSTRUKSI DAN EKSPRESI GEN DNA POLIMERASE MUTAN DELESI BAKTERI TERMOFILIK ISOLAT CIMANGGU DI Escherichia coli

Commercially available thermostable DNA Polymerases possess different properties. Hence, studies on novel thermostable DNA Polymerases are still needed. A thermophilic bacterium, closely related to Bacillus thermoleovorans based on its phylogeny, has been isolated from Cimanggu hot spring (pH 5, 70Â...

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Bibliographic Details
Main Author: Ekawardhani, Savira
Format: Theses
Language:Indonesia
Online Access:https://digilib.itb.ac.id/gdl/view/1875
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Institution: Institut Teknologi Bandung
Language: Indonesia
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Summary:Commercially available thermostable DNA Polymerases possess different properties. Hence, studies on novel thermostable DNA Polymerases are still needed. A thermophilic bacterium, closely related to Bacillus thermoleovorans based on its phylogeny, has been isolated from Cimanggu hot spring (pH 5, 70°C). Whole coding sequence of DNA Polymerase 1 gene from the bacterium has been cloned and sequenced. Since structure-function studies on this thermostable DNA Polymerase require mutant enzymes, therefore the aim of this research was to construct deletion (∆) mutants of polymerase gene which was performed by in frame-deletion method using restrictrion enzyme. The over expressed ∆ mutant genes were constructed in the expression vector (pTrxFus) with tryptophan induced system, identified and sequenced. The mutant enzymes were characterized by SDS-PAGE and its polymerase activities. The mutant enzymes which were constructed in this research indicated the following properties : Mutant ∆EcoRl enzyme lost one of its carboxylate triad, i.e Asp653 Mutant ∆Xhol enzyme lost its 5'-3' and 3'-5' exonuclease domain. Mutant ∆RsaI enzyme lost its N-terminal or the 5'-3' exonuclease domain. Qualitative activity assay on mutant ∆EcoRI (89 kDa) crude extract showed that the mutant lost its polymerase activity compared to its wild type. DNA polymerase mutant ∆Xhol gene was not expressed although the plasmid and the sequence of the gene were still unchanged.

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