Team:Bilkent UNAM Turkey/Experiment

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We ordered our genes. We optimized codon usage because of gene taken from <i>E. cloacae</i>.
+
We ordered synthetic nfsI gene from a company. We optimized codon usage because of gene taken from <i>Enterobacter cloacae</i>.
-
<a href="https://2011.igem.org/Team:Bilkent_UNAM_Turkey/Codon_Optimization"><p>Codon Usage </a>
+
<a href="https://2011.igem.org/Team:Bilkent_UNAM_Turkey/Codon_Optimization"><br>Codon Usage </a>.
 +
We optimized our nfsI gene according to <i>Chlamydomonas reinhardtii</i> codon bias table provided by DNA 2.0. This program enables to change synonymous codons without changing amino acid sequence. You can also check the restriction sites while optimizing codons.  We also avoided from forbidden restriction sites (EcoRI, XbaI, SpeI, PstI) therefore; we have chosen second frequently used codons for 34., 35., 38. and 45. amino acids.
 +
<br>
 +
<img src="https://static.igem.org/mediawiki/2011/1/10/Synthetic_NFSI_for_C.reinhardtii.PNG"width="800" height="400"><br>
 +
1.<b>Gene Designer DNA 2.0.</b><br><br>
 +
 
Then we did <a href="https://2011.igem.org/Team:Bilkent_UNAM_Turkey/Digestion_%28Gel_Electrophoresis%29">restriction digestion and gel electrophoresis</a>.<br>
Then we did <a href="https://2011.igem.org/Team:Bilkent_UNAM_Turkey/Digestion_%28Gel_Electrophoresis%29">restriction digestion and gel electrophoresis</a>.<br>
-
We repeat this step a lot because of failuire.I put right result<br>
+
This image is the best result of our trials<br>
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<img src="https://static.igem.org/mediawiki/2011/2/2f/C.reinhardtii_genler.png" align="center"></img>
+
 
 +
 
 +
<img src="https://static.igem.org/mediawiki/2011/b/b9/C.reinhardtii_nfsI.png" align="center"> <br>
 +
2.<b>The picture of restricted with EcoRI and PstI, nfsI gene.</b><br><br>
 +
 
 +
<img src="https://static.igem.org/mediawiki/2011/1/1f/C.reinhardtii_genes.PNG" align="center"width="900" height="146" > <br>
 +
3.<b>Our nfsI gene design. It contains XhoI and BamHI therefore; we can ligate into pRbcBRL protein expression vector.</b><br><br>
 +
 
 +
<img src="https://static.igem.org/mediawiki/2011/1/11/XhoI_and_BamHI_restriction_digestion_result_nfsI.png" align="center"></img><br>
 +
4.<b>Confirmation of Ligation nfsI gene with pRbcBRL backbone. This pRbcNFSI construct was done because we have received our biobrick prefix and suffix <a href="https://static.igem.org/mediawiki/2011/3/34/MCS.jpg">gene</a> lately as a result of an ordering problem. We need to go on transfection into <i>C. reinhardtii </i> and TNT tolerance and biodegradation capacity of algae</b><br><br>
 +
 
 +
 
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<img src="https://static.igem.org/mediawiki/2011/9/9b/XhoI_and_BamHI_restriction_digestion_result.png" align="center"></img>
 
-
<img src="https://static.igem.org/mediawiki/2011/c/c7/Confirmation_of_Ligation_Products_with_XhoI_and_BamHI_restriction_digestion.png" align="center"></img>
 
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<br>We used standard <a href="http://tools.invitrogen.com/content/sfs/manuals/purelink_quick_gel_extraction_kit_man.pdf">gel purification kit</a>
<br>We used standard <a href="http://tools.invitrogen.com/content/sfs/manuals/purelink_quick_gel_extraction_kit_man.pdf">gel purification kit</a>
Our ligation style is really similar to iGEM's one.<br>
Our ligation style is really similar to iGEM's one.<br>
-
Our one;
+
Our one;<br>
-
<li>insert volume(µl):X</li>
+
insert volume(µl):X<br>
-
<li>Cut Vector Volume(µl):X</li>
+
Cut Vector Volume(µl):X<br>
-
<li>DEPC-water(µl):8,5-2X</li>
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DEPC-water(µl):8,5-2X<br>
-
<li>T4 DNA ligase(µl):0,5</li>
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T4 DNA ligase(µl):0,5<br>
-
<li>Ligation Buffer(µl):1</li>
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Ligation Buffer(µl):1<br>
-
<li>Total Volume(µl):10</li>
+
Total Volume(µl):10<br>
<br>We transformed our plasmid into E.coli with a <a href="http://www.med.nyu.edu/medicine/labs/blaserlab/Protocols/E-coli_competent_cells_protocol_&_transformation.pdf">protocol.</a><br>
<br>We transformed our plasmid into E.coli with a <a href="http://www.med.nyu.edu/medicine/labs/blaserlab/Protocols/E-coli_competent_cells_protocol_&_transformation.pdf">protocol.</a><br>
We used invitrogen <a href="http://tools.invitrogen.com/content/sfs/manuals/purelink_pro96_plasmid_kit_man.pdf">purification kit </a>to get our plasmid.
We used invitrogen <a href="http://tools.invitrogen.com/content/sfs/manuals/purelink_pro96_plasmid_kit_man.pdf">purification kit </a>to get our plasmid.
We sent genes to sequencing and sequencing data should be available on their <a href="http://partsregistry.org/cgi/partsdb/pgroup.cgi?pgroup=iGEM2011&group=Bilkent_UNAM_Turkey">link</a>.
We sent genes to sequencing and sequencing data should be available on their <a href="http://partsregistry.org/cgi/partsdb/pgroup.cgi?pgroup=iGEM2011&group=Bilkent_UNAM_Turkey">link</a>.
-
PCR procedure for GFP amplification from pKScGFP
+
<h2>Polymerase Chain Reaction  of GFP from pKScGFP</h2><p>
 +
 
 +
For 1.0µl of DNA we added,<br>
 +
• 1.0µl of forward primer<br>
 +
• 1.0µl of reverse primer<br>
 +
• 2.5µl of 10X PCR Buffer<br>
 +
• 0.5µl of MgSO4<br>
 +
• 0.5µl of dNTP mix<br>
 +
• 18.375µl of ddH2O<br>
 +
• 0.125µl of Taq polymerase<br>
 +
<p>
 +
Parameters in thermal cycler were chosen as below:<br>
 +
Denaturation is 95oC for 4min<br>
 +
Annealing is 30 cycles:<br>
 +
• 95oC 1min<br>
 +
• 65oC 1min<br>
 +
• 72oC 2min<br>
 +
Extension 72oC for 10min<br>
 +
4oC hold<p>
 +
 
 +
<h3>GFP fusion</h3><br>
 +
GFP fusion with nfsI gene on our Biobrick is our plannned future work.<br>
 +
 
 +
<h3>Restriction Enzyme Digestion</h3><br>
 +
We obtained nfsI gene synthetically with prefix and suffixes. Synthetic nfsI gene was restriction digested via XhoI/BamHI to create sticky ends at prefix and suffixes.<br>
 +
 
 +
We used pRbcRL as our backbone and as an algal expression plasmid. We restriction digested luciferase gene via XhoI/BamHI restriction enzymes and created a cut vector backbone with sticky ends.<br>
 +
 
 +
<h3>DNA ligation</h3><br>
 +
Then we ligated nfsI gene to the cut vector of pRbcRL (pRbc plasmid backbone) with insert:backbone ratios of 10:1, 3:1 and 1:1. All of them gave good results.<p>
 +
 +
For 10:1 nfsI:pRbc ligation tube,<br>
 +
<table border ="1">
 +
<tr><th>Solution <th>Volume (µl)
 +
<tr><td>pRbc backbone<td> 1.7
 +
<tr><td>Insert nfsI<td> 16.1
 +
<tr><td>T4 ligase buffer (10X)<td> 1
 +
<tr><td>T4 DNA ligase<td> 0.5
 +
<tr><td>ddH2O<td> 0.7
 +
<tr><td>Total<td> 20<p>
 +
</table>
 +
For 3:1 nfsI:pRbc ligation tube,
 +
<table border ="1">
 +
<tr><th>Solution<th>Volume (µl)
 +
<tr><td>pRbc backbone<td>1.7
 +
<tr><td>Insert nfsI<td>4.8
 +
<tr><td>T4 ligase buffer (10X)<td>1
 +
<tr><td>T4 DNA ligase <td>0.5
 +
<tr><td>ddH2O <td>2
 +
<tr><td>Total <td>10<p>
 +
</table>
 +
For 1:1 nfsI:pRbc ligation tube,
 +
<table border ="1">
 +
<tr><th>Solution<th> Volume (µl)
 +
<tr><td>pRbc backbone <td>1.7
 +
<tr><td>Insert nfsI <td>1.6
 +
<tr><td>T4 ligase buffer (10X) <td>1
 +
<tr><td>T4 DNA ligase <td>0.5
 +
<tr><td>ddH2O <td>5.2
 +
<tr><td>Total <td>10
 +
</table>
 +
Competent Escherichia coli DH5α were transformed with pRbcnfsI ligated products and plated to LB ampicillin plates. <br>Colonies were collected after overnight incubation at 37oC, and miniculture was started from each colony. Plasmid DNA isolation was performed by using PureLink™ Quick Plasmid Miniprep Kit of InvitrogenTM.<br>
 +
Nanodrop DNA concentrations after minipreps were as below:<p>
 +
<table border ="1">
 +
<tr><th>Nucleic Acid Conc.</th> <th>Unit</th><th>A260</th><th>A280</th><th>260/280</th><th>260/230</th><th>Sample Type</th>
 +
<tr><td>361.4</td><td>ng/µl</td><td>7.228</td><td>4.334</td><td>1.67</td><td>1.82</td><td>DNA</td>
 +
<tr><td>384.9<td> ng/µl<td> 7.698<td> 4.554<td> 1.69<td> 1.82<td> DNA
 +
<tr><td>558.7<td> ng/µl<td> 11.174<td> 7.232<td> 1.55<td> 1.65<td> DNA
 +
</table>
 +
We proceeded to transformation of this plasmids to microalgae. We co-transformed Chlamydomonas reinhardtii to Tris-acetate-phosphate plus neomycine agar plates with pRbcnfsI and pKS-aphVIII-lox plasmid in order to select colonies based on the arginine deficiency in mutant strain cc-425 of Chlamydomonas reinhardtii. Next step was to collect colonies from plate. But due to time constraints we could not obtain colonies from this experiment yet. After collecting colonies, we plan to subculture colonies in the presence of trinitrotoluene (TNT) and check for change in its concentration.<br>
 +
 
 +
 
 +
 
 +
 
 +
 
 +
 
-
For 1µl of DNA, we added,
 
-
1µl of forward primer
 
-
1µl of reverse primer
 
<!-- up to here  -->
<!-- up to here  -->

Latest revision as of 03:25, 22 September 2011

We ordered synthetic nfsI gene from a company. We optimized codon usage because of gene taken from Enterobacter cloacae.
Codon Usage
. We optimized our nfsI gene according to Chlamydomonas reinhardtii codon bias table provided by DNA 2.0. This program enables to change synonymous codons without changing amino acid sequence. You can also check the restriction sites while optimizing codons. We also avoided from forbidden restriction sites (EcoRI, XbaI, SpeI, PstI) therefore; we have chosen second frequently used codons for 34., 35., 38. and 45. amino acids.

1.Gene Designer DNA 2.0.

Then we did restriction digestion and gel electrophoresis.
This image is the best result of our trials

2.The picture of restricted with EcoRI and PstI, nfsI gene.


3.Our nfsI gene design. It contains XhoI and BamHI therefore; we can ligate into pRbcBRL protein expression vector.


4.Confirmation of Ligation nfsI gene with pRbcBRL backbone. This pRbcNFSI construct was done because we have received our biobrick prefix and suffix gene lately as a result of an ordering problem. We need to go on transfection into C. reinhardtii and TNT tolerance and biodegradation capacity of algae


We used standard gel purification kit Our ligation style is really similar to iGEM's one.
Our one;
• insert volume(µl):X
• Cut Vector Volume(µl):X
• DEPC-water(µl):8,5-2X
• T4 DNA ligase(µl):0,5
• Ligation Buffer(µl):1
• Total Volume(µl):10

We transformed our plasmid into E.coli with a protocol.
We used invitrogen purification kit to get our plasmid. We sent genes to sequencing and sequencing data should be available on their link.

Polymerase Chain Reaction of GFP from pKScGFP

For 1.0µl of DNA we added,
• 1.0µl of forward primer
• 1.0µl of reverse primer
• 2.5µl of 10X PCR Buffer
• 0.5µl of MgSO4
• 0.5µl of dNTP mix
• 18.375µl of ddH2O
• 0.125µl of Taq polymerase

Parameters in thermal cycler were chosen as below:
Denaturation is 95oC for 4min
Annealing is 30 cycles:
• 95oC 1min
• 65oC 1min
• 72oC 2min
Extension 72oC for 10min
4oC hold

GFP fusion


GFP fusion with nfsI gene on our Biobrick is our plannned future work.

Restriction Enzyme Digestion


We obtained nfsI gene synthetically with prefix and suffixes. Synthetic nfsI gene was restriction digested via XhoI/BamHI to create sticky ends at prefix and suffixes.
We used pRbcRL as our backbone and as an algal expression plasmid. We restriction digested luciferase gene via XhoI/BamHI restriction enzymes and created a cut vector backbone with sticky ends.

DNA ligation


Then we ligated nfsI gene to the cut vector of pRbcRL (pRbc plasmid backbone) with insert:backbone ratios of 10:1, 3:1 and 1:1. All of them gave good results.

For 10:1 nfsI:pRbc ligation tube,

Solution Volume (µl)
pRbc backbone 1.7
Insert nfsI 16.1
T4 ligase buffer (10X) 1
T4 DNA ligase 0.5
ddH2O 0.7
Total 20

For 3:1 nfsI:pRbc ligation tube,
SolutionVolume (µl)
pRbc backbone1.7
Insert nfsI4.8
T4 ligase buffer (10X)1
T4 DNA ligase 0.5
ddH2O 2
Total 10

For 1:1 nfsI:pRbc ligation tube,
Solution Volume (µl)
pRbc backbone 1.7
Insert nfsI 1.6
T4 ligase buffer (10X) 1
T4 DNA ligase 0.5
ddH2O 5.2
Total 10
Competent Escherichia coli DH5α were transformed with pRbcnfsI ligated products and plated to LB ampicillin plates.
Colonies were collected after overnight incubation at 37oC, and miniculture was started from each colony. Plasmid DNA isolation was performed by using PureLink™ Quick Plasmid Miniprep Kit of InvitrogenTM.
Nanodrop DNA concentrations after minipreps were as below:

Nucleic Acid Conc. UnitA260A280260/280260/230Sample Type
361.4ng/µl7.2284.3341.671.82DNA
384.9 ng/µl 7.698 4.554 1.69 1.82 DNA
558.7 ng/µl 11.174 7.232 1.55 1.65 DNA
We proceeded to transformation of this plasmids to microalgae. We co-transformed Chlamydomonas reinhardtii to Tris-acetate-phosphate plus neomycine agar plates with pRbcnfsI and pKS-aphVIII-lox plasmid in order to select colonies based on the arginine deficiency in mutant strain cc-425 of Chlamydomonas reinhardtii. Next step was to collect colonies from plate. But due to time constraints we could not obtain colonies from this experiment yet. After collecting colonies, we plan to subculture colonies in the presence of trinitrotoluene (TNT) and check for change in its concentration.
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