KONSTRUKSI GEN PENGKODE FARNESYL PYROPHOSPHATE SYNTHASE (FPS), SALAH SATU ENZIM PADA BIOSINTESIS OBAT ANTIMALARIA ARTEMISININ,KE DALAM VEKTOR BINER pCAMBIA 1303
Artemisinin is a secondary metabolite derived from Artemisia annua L. that is effective as anti-malarial drug. However, the level of artemisinin in A. annua is very low and artemisinin-based malaria treatment being relatively expensive. Therefore, an effective strategy to increase the levels of a...
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| Format: | Final Project |
| Language: | Indonesia |
| Online Access: | https://digilib.itb.ac.id/gdl/view/45493 |
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| Institution: | Institut Teknologi Bandung |
| Language: | Indonesia |
| Summary: | Artemisinin is a secondary metabolite derived from Artemisia annua L. that is effective as
anti-malarial drug. However, the level of artemisinin in A. annua is very low and
artemisinin-based malaria treatment being relatively expensive. Therefore, an effective
strategy to increase the levels of artemisinin is needed. Nowadays, researches thus have
been developing leads to genetic engineering involving biosynthetic pathway of
artemisinin. In artemisinin biosynthesis, farnesyl pyrophosphate synthase (FPS) is one of
the enzymes which have an important role. This enzyme will be transform to A. annua in
order to increase the level of artemisinin. To transforms FPS gene in to A. annua, this gene
should be inserted to binary vector pCAMBIA 1303. This study aimedto insert FPS gene
into binary vector pCAMBIA 1303. FPS gene used in this study is a synthetic gene that has
been in the cloning vector pUC57. pUC57-FPS plasmid and empty pCAMBIA plasmid
which has been reproduced were cut using restriction enzymes SpeI and NcoI. Construction
was conducted by ligating two DNA fragments that have been truncated and subsequently
transformed in Escherichia coli strain DH5?. The results showed that FPS gene was
successfully inserted into a vector pCAMBIA 1303, so it produced a recombinant vector
pCAMBIA 1303-FPS. Recombinant vector that has been isolated and analyzed by
electrophoreses using 1% agarose gel and was confirmed by migration analysis, PCR using
specific primers FPS, restriction analysis and determining the nucleotide sequence
(sequencing). Confirmation results showed that recombinant plasmid was migrated slowly,
PCR result showed there is a fragment DNA of FPS on the size of ±1032 bp and this
fragment can be cut by using restriction enzyme XbaI. In the determination of FPS gene
nucleotide sequence (sequencing), the result is not well-confirmed yet.
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