Difference between revisions of "Team:Paris Bettencourt/Notebook/VitaminB2"

Revision as of 16:07, 10 August 2015

13/07

Received gBlocks RibA, RibD, RibE, RibT25 and RibT48 and amplification oligos from IDT.

1 μL gBlock (0.1 to 1ng)
1 μL forward primer (10 μM)
1 μL reverse primer (10 μM)
22 μL DNAse/RNAse free water
25 μL LifeTech MasterMix (2X)

RibA

o15.001

o15.002

RibD

o15.003

o15.004

RibE

o15.005

o15.006

RibT25

o15.007

o15.008

RibT48

o15.009

o15.010

time (min)	temperature (°C)	function
3:00	98	melting

0:30	98	melting
0:30	52	annealing
1:00	72	extension

10:00	72	extension
forever	12	storage

PCR purification protocol

Add 5 volumes of resuspension buffer to 1 volume of PCR product in an 1.5mL microcentrifuge tube, mix by pipetting up and down
Transfer in a centrifugation column
Centrifuge 1 min at 14000 rpm
Throw the filtration product
Add 700μL of washing solution
Centrifuge 1 min at 14000 rpm
Throw the filtration product
Add 500μL of washing solution
Centrifuge 1 min at 14000 rpm
Throw the filtration product
Centrifuge 1 min at 14000 rpm
Throw the filtration product
Put the column in a sterile 1.5mL microcentrifuge tube
Add 45μL of DNAse/RNAse free water on the membrane
Wait 2 minutes
Centrifuge 2min at 10000rpm
Discard the column, DNA is saved in water

Concentrations measured with a Nanodrop:

	[PCR product with gBlock] (ng/μL)	[PCR product without gBlock] (ng/μL)
RibA	3.5	3.4
RibD	6.4	3.3
RibE	5.0	3.7
RibT25	3.5	3.8
RibT48	8.7	3.3

Almost no difference between the PCR and their corresponding negative control.
It could be the fallout of the limited number of cycles. (We only used 12 cycles, as advised by IDT)
NEB Tm calculator gave really different Tm for the PCR primers than Geneious and IDT.
We decided to launch two PCR, both with 35 cycles, but with two different annealing
temperature: 52 and 64°C.

14/07
Launched the two different PCR with different Tm.

PCR with high annealing temperature, 35 cycles:

time (min)	temperature (°C)	function
3:00	98	melting

0:30	98	melting
0:30	64	annealing
1:00	72	extension

10:00	72	extension
forever	12	storage

PCR with low annealing temperature, 35 cycles:

time (min)	temperature (°C)	function
3:00	98	melting

0:30	98	melting
0:30	64	annealing
1:00	72	extension

10:00	72	extension
forever	12	storage

After PCR, we ran the PCR products on a TAE - 1% agarose gel (100V, 20min) to check
if the amplification product correspond to the expected size of the gBlocks.

From left to right:
1kb Ladder, RibA, D, E, T25 and T48 amplified at 52°C
and Rib A, D, E, T25 and T48 amplified at 64°C

The bands are not really specific and seems to be smeared over the gel.
However, we can see that the extremity of each band correspond approximatively
to the expected size of our parts, except RibD amplified at 64°C for which no band has been detected. We purified our PCR product according to the previously used protocol,
and then measure the DNA concentration using a Nanodrop.

Part Name	PCR product amplified at 52°C concentration (ng/μL)	PCR product amplified at 64°C concentration (ng/μL)
RibA	54.3	132.7
RibD	50.5	140.2
RibE	67.1	78.2
RibT25	63.6	136.0
RibT48	61.2	143.1

16/07
Annealing of o15.011 (TCGACCATGCTTGTCTTCGAAGACTTGGGGGAT) and o15.012 (CTAGATCCCCCAAGTCTTCGAAGACAAGCATGG) using the following protocol:

Annealing Protocol

Phosphorylation of the oligos
- 5.6μL DNAse/RNAse free water
- 6.0μL o15.011 (10µM)
- 6.0μL o15.012 (10µM)
- 2.0μL 10X T4 DNA ligase buffer
- 0.4μL T4 PolyNucleotide Kinase Total: 20μL
incube 30min at 37°C
add 1μL of 1M NaCl
incube 5min at 95°C
let the mix cool down
use 2μL of the mix as a 10X solution

Inoculate LB + erythromycin (150ng/μL) with g15.21 containing pKV6.
Inoculate M17 + erythromycin (10ng/μL) with g15.13 containing pSIP411.

@@ Line 270: / Line 270: @@
    <tr>
      <td><i>From left to right:<br/>
-<i>1kb Ladder, RibA, D, E, T25 and T48 amplified at 52°C <br/>
+      <i>1kb Ladder, RibA, D, E, T25 and T48 amplified at 52°C <br/>
-and Rib A, D, E, T25 and T48 amplified at 64°C<i>
+      and Rib A, D, E, T25 and T48 amplified at 64°C<i>
      </td>
    </tr>
 </table>
+<br/>
+The bands are not really specific and seems to be smeared over the gel.<br/>
+However, we can see that the extremity of each band correspond approximatively <br/>
+to the expected size of our parts, except RibD amplified at 64°C for which no band has been detected.
+We purified our PCR product according to the previously used protocol,<br/>
+and then measure the DNA concentration using a Nanodrop.
+<table style="width:25%">
+  <tr>
+    <td><b>Part Name </b></td>
+    <td><b>PCR product amplified at 52°C concentration (ng/μL)</b></td>
+    <td><b>PCR product amplified at 64°C concentration (ng/μL) </b></td>
+  </tr>
+  <tr>
+    <td>RibA</td>
+    <td>54.3</td>
+    <td>132.7</td>
+  </tr>
+  <tr>
+    <td>RibD</td>
+    <td>50.5</td>
+    <td>140.2</td>
+  </tr>
+  <tr>
+    <td>RibE</td>
+    <td>67.1</td>
+    <td>78.2</td>
+  </tr>
+  <tr>
+    <td>RibT25</td>
+    <td>63.6</td>
+    <td>136.0</td>
+  </tr>
+  <tr>
+    <td>RibT48</td>
+    <td>61.2</td>
+    <td>143.1</td>
+  </tr>
+</table>
+<br/><b>16/07</b><br/>
+Annealing of o15.011 (TCGACCATGCTTGTCTTCGAAGACTTGGGGGAT) and o15.012 (CTAGATCCCCCAAGTCTTCGAAGACAAGCATGG) using the following protocol:
+<br/>
+<table>
+  <tr>
+    <td>Annealing Protocol
+<ul>
+<li>Phosphorylation of the oligos
+<ul>
+  <li>        5.6μL	DNAse/RNAse free water
+  <li>	6.0μL   o15.011 (10µM)
+  <li>	6.0μL   o15.012 (10µM)
+  <li>	2.0μL   10X T4 DNA ligase buffer
+  <li>	0.4μL   T4 PolyNucleotide Kinase
+Total:   20μL
+</ul>
+<br/>
+  <li>incube 30min at 37°C
+  <li>add 1μL of 1M NaCl
+  <li>incube 5min at 95°C
+  <li>let the mix cool down
+  <li>use 2μL of the mix as a 10X solution
+</ul>
+    </tr>
+  </td>
+</table>
+<br/>
+Inoculate LB + erythromycin (150ng/μL) with g15.21 containing pKV6.<br/>
+Inoculate M17 + erythromycin (10ng/μL) with g15.13 containing pSIP411.