Team:KAIST-Korea/Project/Methods
From 2010.igem.org
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STAT<br> | STAT<br> | ||
We need two kinds of brick to do PCR. One is STAT and the other is V_STAT. STAT would be cut by EcoRI and inserted into pBS1C3 for the submission. V_STAT would be cut by NdeI and BamHI sites and inserted into pREP41 vector for the expression<br> | We need two kinds of brick to do PCR. One is STAT and the other is V_STAT. STAT would be cut by EcoRI and inserted into pBS1C3 for the submission. V_STAT would be cut by NdeI and BamHI sites and inserted into pREP41 vector for the expression<br> | ||
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Fusion Antibody Receptor<br> | Fusion Antibody Receptor<br> | ||
[[Image:FAR.jpg|center]]<br> | [[Image:FAR.jpg|center]]<br> | ||
We need six bricks to do PCR. They are B_FGFR, F_FGFR, SIG, IG, SIG + IG, and Ab. B_FGFR is a orignal back part of FGFR to operate our system, and F_FGFR is a handdled front part of FGFR assembled our biobrick. SIG is a signal peptide, and IG is IG-like-1, Ab is IG-like-2,and 3 we use. We will use B_FGFR and F_FGFR for the expression and not only these but also the others for the submission.<br> | We need six bricks to do PCR. They are B_FGFR, F_FGFR, SIG, IG, SIG + IG, and Ab. B_FGFR is a orignal back part of FGFR to operate our system, and F_FGFR is a handdled front part of FGFR assembled our biobrick. SIG is a signal peptide, and IG is IG-like-1, Ab is IG-like-2,and 3 we use. We will use B_FGFR and F_FGFR for the expression and not only these but also the others for the submission.<br> | ||
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Homologous Recombination<br> | Homologous Recombination<br> | ||
[[Image:HR.jpg|center]]<br> | [[Image:HR.jpg|center]]<br> | ||
- | We need five bricks to do PCR. They are Fusion Antibody Receptor, 5' UTR-Receptor, 5' UTR-Receptor + Selection marker, 5' UTR-Recptor + Selection Marker + 3' UTR, and Homologous Recombination. Fusion antibody receptor needs to be linked together with UTR and selection marker in order to be inserted into genome by homologous recombination. "Homologous Recombination" is inserted into genome by homologous recombination.<br> | + | We need five bricks to do PCR. They are Fusion Antibody Receptor, 5' UTR-Receptor, 5' UTR-Receptor + Selection marker, 5' UTR-Recptor + Selection Marker + 3' UTR, and Homologous Recombination. Fusion antibody receptor needs to be linked together with UTR and selection marker in order to be inserted into genome by homologous recombination. "Homologous Recombination" is inserted into genome by homologous recombination.<br><br> |
GAS promoter + GFP<br> | GAS promoter + GFP<br> | ||
- | [[Image:Gas.jpg|center| | + | [[Image:Gas.jpg|center|350px]]<br> |
We need three bricks to do PCR. They are Proximal Promoter, Core Promoter+GFP, and PstI+Proximal Promoter+Core Promoter+GFP+NdeI. PstI and NdeI are restiriction enzymes, and Proximal + Core promoter is GAS promoter to express GFP | We need three bricks to do PCR. They are Proximal Promoter, Core Promoter+GFP, and PstI+Proximal Promoter+Core Promoter+GFP+NdeI. PstI and NdeI are restiriction enzymes, and Proximal + Core promoter is GAS promoter to express GFP | ||
Revision as of 08:28, 4 September 2010
Cloning PlanAim
PCR To manipulate gene products obtained from gene-bank, our team used PCR/Real-Time PCR methods. Commercially obtained genes contain few more base pairs added at front and back site. As for FGPR, the receptor protein of human has human-specific signal peptide at its starting point, and this region had to be replaced by S.pombe specific signal peptide to express the protein at membrane region. To do this, PCR primers containing signal peptide region of S.pombe were synthesized by method describeds below. Then, FGPR gene was amplified by PCR to get gene product whose signal region is replaced. Also, additional sequence at rear site of gene was removed. STAT gene went through similar process; removing additional region. We need six bricks to do PCR. They are B_FGFR, F_FGFR, SIG, IG, SIG + IG, and Ab. B_FGFR is a orignal back part of FGFR to operate our system, and F_FGFR is a handdled front part of FGFR assembled our biobrick. SIG is a signal peptide, and IG is IG-like-1, Ab is IG-like-2,and 3 we use. We will use B_FGFR and F_FGFR for the expression and not only these but also the others for the submission. We need five bricks to do PCR. They are Fusion Antibody Receptor, 5' UTR-Receptor, 5' UTR-Receptor + Selection marker, 5' UTR-Recptor + Selection Marker + 3' UTR, and Homologous Recombination. Fusion antibody receptor needs to be linked together with UTR and selection marker in order to be inserted into genome by homologous recombination. "Homologous Recombination" is inserted into genome by homologous recombination. GAS promoter + GFP We need three bricks to do PCR. They are Proximal Promoter, Core Promoter+GFP, and PstI+Proximal Promoter+Core Promoter+GFP+NdeI. PstI and NdeI are restiriction enzymes, and Proximal + Core promoter is GAS promoter to express GFP
Oligo Synthesis Oligo-synthesis was supported by Bioneer. Codon optimization Oligo Design S/W
Mega-base Oligo Synthesizer
AccuRapid Cell-Free Protein Expression Kit
Gene Synthesis Kit
Homologous Recombination Homologous recombination is a type of genetic recombination in which nucleotide sequences are exchanged between two similar or identical molecules of DNA. It is most widely used by cells to accurately repair harmful breaks that occur on both strands of DNA, known as double-strand breaks. Homologous recombination also produces new combinations of DNA sequences during meiosis, the process performed by many eukaryotes like animals and plants: production of sperm and egg cells. These new combinations of DNA promote genetic variations in offspring, which in turn enable populations to evolve. Homologous recombination is also used in horizontal gene transfer to exchange genetic material between different strains and species of bacteria and viruses.
TA cloning TA cloning is one of the subcloning techniques. This technique starts from product of PCR that uses taq DNA polymerase. Taq DNA polymerase tends to add one adenine overhang to the 3` end of PCR product. This result occurs because there is lack of ability to proofread from 3` to 5`. Therefore after PCR process, we can get amplified DNA sequences that has single adenine overhang on 3` end.
ReferencesBioneer PCR service: |