CLONING AND HETEROLOGOUS EXPRESSION OF PATATIN LIKE PHOSPHOLIPASE GENE FROM LOCAL ISOLATE AL17
Patatin-like phospholipase is an enzyme that plays a role in hydrolyzing phospholipid ester bonds. Local isolate AL17 is known to contain a gene encoding patatin-like phospholipase. This study focuses on obtaining patatin-like phospholipase from the AL17 and characterize its properties. The re...
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| Format: | Theses |
| Language: | Indonesia |
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| Online Access: | https://digilib.itb.ac.id/gdl/view/87415 |
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| Institution: | Institut Teknologi Bandung |
| Language: | Indonesia |
| Summary: | Patatin-like phospholipase is an enzyme that plays a role in hydrolyzing
phospholipid ester bonds. Local isolate AL17 is known to contain a gene encoding
patatin-like phospholipase. This study focuses on obtaining patatin-like
phospholipase from the AL17 and characterize its properties. The research was
conducted in four main steps, namely gene cloning, bioinformatics and
biocomputation analysis of the gene, expression, and characterization of the
enzyme. For the gene cloning, two specific primer pairs were designed to amplify
the target genes from the bacterial genome. The amplification results obtained two
gene fragments, namely patatin-like phospholipase 1 (ITBPLP1) and patatin-like
phospholipase 2 (ITBPLP2), with the size of 2,3 and 1.1 kb, respectively. These
gene fragments were then ligated to cloning vectors, resulting in recombinant
plasmids, namely pJET-ITBPLP1 and pJET-ITBPLP2, used for transformation of
Escherichia coli TOP10. The plasmids were further analyzed through sequencing
and bioinformatics. The sequence was translated to amino acids, which showed the
presence of four important conserved regions. In addition, the sequence showed
similarity levels at 46% and 39% to similar genes from Pseudomonas aeruginosa.
For the expression, the genes were reamplified using expression primers containing
NdeI and SalI. Following the amplification, the amplicons were inserted to
pET30a(+) at the NdeI and SalI restriction site, resulting pET-ITBPLP1.1, pET
ITBPLP1.2, and pET-ITBPLP2. The combined expression vectors were used to
transform Escherichia coli BL21 (DE3). The genes were expressed on Luria
Bertani at 37 °C by induction of IPTG. The proteins were isolated using the alkaline
lysis method with 0.1% SDS. Following SDS-PAGE, ITBPlp1.1 and ITBPlp1.2
were overexpressed, while ITBPlp2 was expressed at a low level. All the three
enzymes exhibited hydrolysis activity on para-nitrophenyl decanoate. In silico
characterization using molecular docking showed that the enzyme ITBPlp1 prefer
para-nitrophenyl butyrate, while ITBPlp2 prefer para-nitrophenyl decanoate. |
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