Difference between revisions of "Team:USP-EEL-Brazil/Experiments"
PedroAlmeida (Talk | contribs) |
PedroAlmeida (Talk | contribs) |
||
| Line 69: | Line 69: | ||
<img style="text-align:center;"src="https://static.igem.org/mediawiki/2018/0/08/T--USP-EEL-Brazil--eembbrazil.jpg"width=100% > | <img style="text-align:center;"src="https://static.igem.org/mediawiki/2018/0/08/T--USP-EEL-Brazil--eembbrazil.jpg"width=100% > | ||
| − | <div class="margin" style=" margin-bottom: 100px; text-align: justify; text-indent: | + | <div class="margin" style=" margin-bottom: 100px; text-align: justify; text-indent: 3%; "> |
<p>Experimentos</p> | <p>Experimentos</p> | ||
Revision as of 21:47, 11 October 2018
Experimentos
Molecular Biology
The molecular biology stage is the initial part of our project in relation to LabWork. To obtain the enzyme of interest, laccase, the following steps must be taken:
- Amplification of gene (PCR); (seria legal se cada um desses tópicos fossem redirecionados para os respectivos protocolos)
- Gene cloning (3A Assemlby);
- Bacterial transformation;
- Expression and purification of enzyme;
Here we will address the steps of amplification, cloning and transformation. To carry out the experiments you need the genetic material (primers, promoters, RBSs, genes, terminators, vectors, etc)
The genes we are working on, LacPL and LacPH, are constituted of RBS (BBa_0030) and CDS. The promoter and the terminator were used of BBa_R0010 (Kit plate 3 Well 4G). The cloning was made inserting the genes into the BBa_R0010.
Our DNA was synthetized in gBlock format by IDT.
imagemOur synthetic DNA were synthetized in gBlocks. For the gene to become functional we did Gibson Assembly to lligate the gBlocks.
imagemCOnfirmed the Gibson assembly we amplified the Gibson products by PCR.
imagemMade the amplification of genes, we prepared the vector with LacI promoter (BBa_R0010) and linearized plasmide backbone pSB1C3 (2016) for insertion of genes. The BBa_R0010 was transformaded in DH5alpha for production of more plasmids.
imagemWith the plasmids and the genes ready, we did 3A Assembly to insert our gene. First, we inserted the gene into linearized plasmid pSB1C3 from USP-EEL BRAZIL Team 2016, because we do not have the DpnI enzyme. For this reason, we tried insert also into BBa_J04450
imagem imagemSimultaneously, we did 3A Assembly for insertion of the gene into BBa_R0010. The 3A Assembly protocol was modified as following: The part “A” was cleaved using SpeI and PstI and the gene was cleaved by Xbal and Pstl. By making the ligation, the site for part A’s Spel ligate to the site of the Xbal of our gene, making he “M” point. Then the Pstl’s site of the plasmid of our gene ligate and close the plasmid.
imagemAfter this ligation step, it was transformed in E. coli DH5alpha and we did the colony PCR.
imagem imagem imagemLooking at the results, we can confirm that the genes are in the colony with the gene LacPL in BBa_R0010 (Lacl promoter) and LacPL in the linearized vector and also LacPH in BBa_J04450.
Expression and Purification
Get in touch, or swing by for a cup of coffee.
Biochemical Characterization
Get in touch, or swing by for a cup of coffee.