Team:HUST-China/Protocol/Part1
From 2013.igem.org
JianhaoZeng (Talk | contribs) |
JianhaoZeng (Talk | contribs) |
||
(8 intermediate revisions not shown) | |||
Line 90: | Line 90: | ||
</tr> | </tr> | ||
<tr class="success"> | <tr class="success"> | ||
- | <td> | + | <td>pET-28a(+)</td> |
<td>vectors</td> | <td>vectors</td> | ||
<td>conserved in the lab</td> | <td>conserved in the lab</td> | ||
Line 188: | Line 188: | ||
<tr class="success"> | <tr class="success"> | ||
<th width="10px">Item</th> | <th width="10px">Item</th> | ||
- | <th>System components(50μl) | + | <th>System components(50μl)</th> |
- | + | ||
</tr> | </tr> | ||
</thead> | </thead> | ||
<tbody> | <tbody> | ||
<tr class="success"> | <tr class="success"> | ||
- | <td>Solution I | + | <td>Solution I </td> |
- | <td> | + | <td>5ul</td> |
</tr> | </tr> | ||
<tr class="success"> | <tr class="success"> | ||
- | <td>DNA | + | <td>DNA </td> |
- | + | ||
- | + | <td>4.5ul</td> | |
+ | </tr> | ||
<tr class="success"> | <tr class="success"> | ||
- | <td>pMD18T 0. | + | <td>pMD18T </td> |
- | + | <td>0.5ul</td> | |
- | </tr> | + | </tr> |
+ | <th>Conditions</th> | ||
+ | <td> 16℃ 2h</td> | ||
+ | </tr> | ||
</tbody> | </tbody> | ||
</table> | </table> | ||
Line 234: | Line 237: | ||
<p class="small">Fig1-5 (araC-O,araC,M5000,P-O,P)</p> | <p class="small">Fig1-5 (araC-O,araC,M5000,P-O,P)</p> | ||
</div> | </div> | ||
- | <p><strong>Step 5 : </strong>The novel plasmid was transferred into BL21strain, which later was grew in the Amp+ LB broth, | + | <p><strong>Step 5 : </strong>The novel plasmid was transferred into BL21strain, which later was grew in the Amp+ LB broth, 37℃ for one night. To ensure the conjunctions were correct, we confirmed the vectors by colonial PCR and gel electrophoresis, following the digestion of SpeI and PstI to see the possibilities of reverse connection. It was proven that one out of 10 mono-clones we picked was in the right in the marker ladder but reverse connected in the plasmid. So we picked mono-colonies and testified again and again to harvest correct plasmid in considerable concentration. (See fig1-6) The conditions for gene conjunction/ colonial PCR / dual-enzyme digestion reaction were listed in the table 1-6,1-7,1-8. |
</p> | </p> | ||
<table class="table table-condensed table-hover table-bordered" style="background:#fffdfd"> | <table class="table table-condensed table-hover table-bordered" style="background:#fffdfd"> | ||
Line 249: | Line 252: | ||
<td>1</td> | <td>1</td> | ||
<td>Solution I 5μl </td> | <td>Solution I 5μl </td> | ||
- | <td> | + | <td></td> |
</tr> | </tr> | ||
<tr class="success"> | <tr class="success"> | ||
Line 259: | Line 262: | ||
<td>3</td> | <td>3</td> | ||
<td>pMD18T 0.5μl</td> | <td>pMD18T 0.5μl</td> | ||
- | <td> | + | <td></td> |
</tr> | </tr> | ||
</tbody> | </tbody> |
Latest revision as of 16:16, 28 October 2013
The construction of the biological oscillator
·Materials
Strains and vectors | Relevant genotype and characteristics | Originate |
---|---|---|
E.coli DH5 α | strains | conserved in the lab |
pET-28a(+) | vectors | conserved in the lab |
pSB1C3 vectors | vectors | conserved in the lab |
·Methods
Step 1 : To find the optimal temperature for araC amplification, we set a gradient in temperature . Then we amplified araC sequence by PCR in 58.5℃. The sequence was stored in -20℃. The PCR conditions were listed as table 1-3.
System components(30μl) | Volume |
---|---|
ddH2O | 17.1 |
PrimerStar Buffer | 6 |
dNTP | 3 |
PR | 1.5 |
PF | 1.5 |
Template | 0.6 |
TPrimerStar | 0.3 |
Step 2 : Digest 2118CA vector(fig1-1) to dismiss its original promoter and 2512EA vector(fig1-2) to donate a hybrid promoter with EcoR I and SpeI. Retrieve and purify the target genes with kits produced by. fig1-3 was the gel image of the skeleton and hybrid promoter. Afterwards,2118CA’s skeleton and hybrid promoter were linked together to recombine a new vector:2118CA+hp. The conditions for gene digest and conjunction were listed in the table 1-4,1-5.
System components(50μl) | Conditions |
---|---|
10×H Buffer 5μl | 37℃ 1h |
EocRI 2.5μl | 37℃ 1h |
PstI 2.5μl 10μl | 37℃ 1h |
ddH2O up to 50μl | 37℃ 1h |
Item | System components(50μl) |
---|---|
Solution I | 5ul |
DNA | 4.5ul |
pMD18T | 0.5ul | Conditions | 16℃ 2h |
Fig1-1 structure of 2118CA
Fig1-2 structure of 2512EA
Fig1-3 Gel images of enzyme digest of 2118CA and 2512CA
Step 3 : To verify the linking reaction was correct, we had the conjunct gene digested with EcoR I and SpeI, following that we loaded the 2118CA+hp plasmid in the agarose gel electrophoresis. The final image was displaced in fig1-4.
Fig1-4 Verification of 2118CA+hp plasmid(1.2118CA+hp 2,1,O,M5000)
Step 4 : Dispose previous araC gene sequence with XbaI and SpeI to expose the restriction enzyme site at both terminals. Digest 2118CA+hp plasmid with Spel to create an incision for inserting araC fragment. After verifying two fragments using agarose gel electrophoresis(fig1-5), they were linked together creating the active feedback part.
Fig1-5 (araC-O,araC,M5000,P-O,P)
Step 5 : The novel plasmid was transferred into BL21strain, which later was grew in the Amp+ LB broth, 37℃ for one night. To ensure the conjunctions were correct, we confirmed the vectors by colonial PCR and gel electrophoresis, following the digestion of SpeI and PstI to see the possibilities of reverse connection. It was proven that one out of 10 mono-clones we picked was in the right in the marker ladder but reverse connected in the plasmid. So we picked mono-colonies and testified again and again to harvest correct plasmid in considerable concentration. (See fig1-6) The conditions for gene conjunction/ colonial PCR / dual-enzyme digestion reaction were listed in the table 1-6,1-7,1-8.
Item | System components(50μl) | Conditions |
---|---|---|
1 | Solution I 5μl | |
2 | DNA 4.5μl | 16℃ 2h |
3 | pMD18T 0.5μl |
Item | System components(50μl) | Conditions |
---|---|---|
1 | 2×EX Tag Mix 5μl | 94℃5min |
2 | M13-47(10μmol/L)0.5μl | 94℃30sec |
3 | M13-48(10μmol/L)0.5μl | 58℃30sec |
4 | ddH2O up to 10μl | 72℃(1min for ygfG, ygfD 1min30sec for ygfH 2min for Sbm) 10min |
Fig1-6 we tried four times to find out the positive plasmid
Step 6 : After successfully constructing the active part of the dual-feedback oscillator, we engaged to build the repressor part, pET28 vector with a replaced lacI structural gene and a hybrid promoter. As the sequences of original lacI in pET28 have the restriction recognizing sites namely Mul I and BssH II, we chose the way of digestion by these two enzymes to dismiss the original lacI. Then we did the next gene conjunction to introduce hybrid promoter and a new lacI gene on condition that the previous result was validated. The general operations were similar, so there should be a reasonable ellipsis.
Step 7 : Even we had our oscillator constructed, to coherent with the modeling mates’ opinion, we added LAA tags to the end of araC and rfp reporter gene to accelerate degradation. To increase the transformation percent, we cut the sequence of hybrid-araC-LAA-rfp-LAA from 2118CA and pasted on pET28 vector.