Revision as of 01:08, 18 October 2014

Exeter | ERASE

Lab Book

On this page you can find out more about how our project progressed over time. Our data was originally written in a standard lab book. We have scanned in each page of the book. Each page is listed with along with the page number, the date the page covers, a short description of work carried out that day as well as who did it.

Page No.	Date:	Description:	Carried out by:
1	30/06/14	Transformation of iGEM standardised DNA into plasmids for culturing. RBSs and protocols listed.	Martyn Bennet, Beth Hickton
2	31/06/14	Transformation of iGEM DNA into plasmids for culturing, cont. List of promoters transformed./td>	Beth Hickton, Edward Muir
3	01/07/14	List of promoters transformed, cont. Transformations were plated.	Beth Hickton, Martyn Bennet
4	02/07/14	The previous day transformations were plated.	Beth Hickton
5	02/07/14	Transformation of iGEM re-suspended promoters.	Beth Hickton
6	02/07/14	Preparation of competent E. coli cells	Beth Hickton
7	03/07/14	Promoter transformation results.	Jessica Rollit, Martyn Bennet
8	03/07/14	E. coli growth rate.	Edward Muir, Beth Hickton
9	04/07/14	Transformation of promoters and gene constructs.	Edward Muir, Beth Hickton
10	07/07/14	Putting constructs into the iGEM vector and testing for transformation efficiency.	Martyn Bennet, Edward Muir, Beth Hickton
11	08/07/14	Repeat construct addition into iGEM vector and testing transformation efficiency.	Edward Muir, Beth Hickton, Martyn Bennet
12	08/07/14	Transforming constructs into Top10 and DH5.	Beth Hickton, Martyn Bennet, Edward Muir
13	09/07/14	Results of Construction of iGEM vector.	Jessica Rollit, Beth Hickton
14	10/07/14	A range of mini-preps	Jessica Rollit, Beth Hickton
15	11/07/14	Measuring the length of DNA.	Edward Muir
16	11/07/14	Measuring the length of DNA, cont.	Edward Muir
17	11/07/14	Mini-prepping picked cultures containing promoters.	Callum Bailey, Elize Hernandez
18	11/07/14	Parts sent for sequencing	Callum Bailey, Elize Hernandez
19	11/07/14	Linearizing DNA.	Edward Muir
20	11/07/14	Creating glycerol stocks.	Beth Hickton, Max Smart
21	14/07/14	GFP and RFP resuspension and transformation.	Edward Muir, Martyn Bennet, Beth Hickton
22	14/07/14	GFP and RFP resuspension and transformation, cont.	Beth Hickton, Edward Muir
23	16/07/14	Mini-prepping GFP and RFP.	Jessica Rollit, Edward Muir, Fran Penrose
24	16/07/14	GFP and RFP digestion/ligation to PSB1C3.	Beth Hickton, Edward Muir
25	16/07/14	Plasmid digestions.	Edward Muir, Callum Bailey, Benjamin Miller
26	16/07/14	RFP/GFP ligations.	Edward Muir
27	16/07/14	RFP/GFP ligations, cont.	Edward Muir
28	17/07/14	Transformation of GFP/RFP with terminator.	Edward Muir
29	18/07/14	Making LB agar for promoters experiment.	Katie Pearce
30	18/07/14	Promoter experiment – quantities.	Edward Muir
31	18/07/14	Promoter experiment – quantities, cont.	Edward Muir
32	18/07/14	Promoter experiment – quantities, cont. 2.	Edward Muir
33	21/07/14	Promoter experiment preliminary timetable.	Edward Muir
34	22/07/14	Electrophoresis of RFP and GFP (with terminators).	Edward Muir
35	22/07/14	Preparation of competent E. coli cells.	Beth Hickton, Peter Reader
36	23/07/14	GFP/RFP + terminator liquid broths mini-prepped.	Beth Hickton, Peter Reader, Jessica Rollit
37	23/07/14	Potassium Chromate preparation.	Peter Reader, Benjamin Miller, Beth Hickton
38	23/07/14	Transformation of other promoters.	Edward Muir
39	24/07/14	Moving GFP+T and RFP+T onto AMP backbones.	Edward Muir, Katie Pearce
40	24/07/14	Ligation of GFP+T and RFP+T onto AMP backbones.	Edward Muir, Beth Hickton
41	24/07/14	Potassium Dichromate colorimetry and spectrophotometry.	Beth Hickton, Edward Muir
42	28/07/14	Plating Anderson RBSs.	Beth Hickton, Edward Muir, Elize Hernandez
43	28/07/14	Mini-prep of reporters, promoters and RBSs.	Beth Hickton, Elize Hernandez, Edward Muir
44	29/07/14	COSHH Form created for Nitroglycerine experiments.	Beth Hickton, Peter Reader, Benjamin Miller
45	30/07/14	Cr(VI) / Ligand experimentation.	Peter Reader
46	31/07/14	Mini-prep of constructs.	Edward Muir, Elize Hernandez, Beth Hickton
47	31/07/14	Digestion and ligation of promoter/RBS combos.	Edward Muir, Callum Bailey
48	31/07/14	Oligo preparation.	Edward Muir, Callum Bailey
49	31/07/14	Ligation of promoter and RBs digestions.	Edward Muir, Callum Bailey, Benjamin Miller
50	01/08/14	Digestion and Ligation of constructs 004 and 007.	Edward Muir, Jessica Rollit, Beth Hickton
51	01/08/14	Digestion and Ligation of constructs 004 and 007, cont.	Edward Muir
52	05/08/14	Colonies picked and mini-prepped.	Callum Bailey
53	05/08/14	Colonies picked and mini-prepped, cont.	Callum Bailey
54	06/08/14	Testing promoter/RBS combination efficiency.	Callum Bailey, Edward Muir
55	06/08/14	Testing promoter/RBS combination efficiency, cont.	Callum Bailey, Edward Muir
56	07/08/14	Picking colonies from promoter/RBS combination transformations.	Edward Muir, Callum Bailey
57	07/08/14	T. Cam experiment.	Edward Muir, Callum Bailey
58	11/08/14	Promoter/RBS combinations again.	Edward Muir, Callum Bailey
59	11/08/14	Promoter/RBS combinations again, cont.	Edward Muir, Callum Bailey
60	11/08/14	Inoculation of enzymes for construct 001 and 003.	Edward Muir, Callum Bailey
61	12/08/14	Inoculation of enzymes for construct 001 and 003, cont.	Edward Muir, Callum Bailey
62	12/08/14	Transformation of a sample promoter/RBS combination.	Callum Bailey
63	12/08/14	T. Cam experiment for solvents and ether.	Edward Muir
64	13/08/14	Combination transformation results and construct testing.	Edward Muir
65	13/08/14	Putting oligos into GFP and RFP.	Edward Muir

These lab book photos are a record of how we produced our synthetic bacterium. All experiments after this point are recorded in their relevant lab reports.

Exeter | ERASE

@@ Line 21: / Line 21: @@
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%281%29_.JPG | 1]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%281%29_.JPG”>1</a></td>
    <td>30/06/14</td> <!-- date -->
    <td>Transformation of iGEM standardised DNA into plasmids for culturing. RBSs and protocols listed.</td>  <!-- desciption -->
@@ Line 27: / Line 27: @@
 </tr>
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-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%282%29_.JPG | 2]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%282%29_.JPG”>2</a></td>
    <td>31/06/14</td>
    <td>Transformation of iGEM DNA into plasmids for culturing, cont. List of promoters transformed./td>
@@ Line 33: / Line 33: @@
 </tr>
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-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%283%29_.JPG | 3]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%283%29_.JPG”>3</a></td>
    <td>01/07/14</td>
    <td>List of promoters transformed, cont. Transformations were plated.</td>
@@ Line 39: / Line 39: @@
 </tr>
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-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%284%29_.JPG | 4]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%284%29_.JPG”>4</a></td>
    <td>02/07/14</td>
    <td>The previous day transformations were plated. </td>
@@ Line 45: / Line 45: @@
 </tr>
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-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%285%29_.JPG | 5]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%285%29_.JPG”>5</a></td>
    <td>02/07/14</td>
    <td>Transformation of iGEM re-suspended promoters.</td>
@@ Line 51: / Line 51: @@
 </tr>
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-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%286%29_.JPG | 6]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%286%29_.JPG”>6</a></td>
    <td>02/07/14</td>
    <td>Preparation of competent E. coli cells</td>
@@ Line 57: / Line 57: @@
 </tr>
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-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%287%29_.JPG | 7]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%287%29_.JPG”>7</a></td>
    <td>03/07/14</td>
    <td>Promoter transformation results.</td>
@@ Line 63: / Line 63: @@
 </tr>
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-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%288%29_.JPG | 8]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%288%29_.JPG”>8</a></td>
    <td>03/07/14</td>
    <td>E. coli growth rate.</td>
@@ Line 69: / Line 69: @@
 </tr>
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-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%289%29_.JPG | 9]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%289%29_.JPG”>9</a></td>
    <td>04/07/14</td>
    <td>Transformation of promoters and gene constructs.</td>
@@ Line 75: / Line 75: @@
 </tr>
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-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2810%29_.JPG | 10]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2810%29_.JPG”>10</a></td>
    <td>07/07/14</td>
    <td>Putting constructs into the iGEM vector and testing for transformation efficiency.</td>
@@ Line 81: / Line 81: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2811%29_.JPG | 11]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2811%29_.JPG”>11</a></td>
    <td>08/07/14</td>
    <td>Repeat construct addition into iGEM vector and testing transformation efficiency.</td>
@@ Line 87: / Line 87: @@
 </tr>
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-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2812%29_.JPG | 12]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2812%29_.JPG”>12</a></td>
    <td>08/07/14</td>
    <td>Transforming constructs into Top10 and DH5.</td>
@@ Line 93: / Line 93: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2813%29_.JPG | 13]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2813%29_.JPG”>13</a></td>
    <td>09/07/14</td>
    <td>Results of Construction of iGEM vector.</td>
@@ Line 99: / Line 99: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2814%29_.JPG | 14]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2814%29_.JPG”>14</a></td>
    <td>10/07/14</td>
    <td>A range of mini-preps</td>
@@ Line 105: / Line 105: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2815%29_.JPG | 15]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2815%29_.JPG”>15</a></td>
    <td>11/07/14</td>
    <td>Measuring the length of DNA.</td>
@@ Line 111: / Line 111: @@
 </tr>
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-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2816%29_.JPG | 16]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2816%29_.JPG”>16</a></td>
    <td>11/07/14</td>
    <td>Measuring the length of DNA, cont.</td>
@@ Line 117: / Line 117: @@
 </tr>
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-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2817%29_.JPG | 17]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2817%29_.JPG”>17</a></td>
    <td>11/07/14</td>
    <td>Mini-prepping picked cultures containing promoters.</td>
@@ Line 123: / Line 123: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2818%29_.JPG | 18]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2818%29_.JPG”>18</a></td>
    <td>11/07/14</td>
    <td>Parts sent for sequencing</td>
@@ Line 129: / Line 129: @@
 </tr>
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-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2819%29_.JPG | 19]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2819%29_.JPG”>19</a></td>
    <td>11/07/14</td>
    <td>Linearizing DNA.</td>
@@ Line 135: / Line 135: @@
 </tr>
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-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2820%29_.JPG | 20]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2820%29_.JPG”>20</a></td>
    <td>11/07/14</td>
    <td>Creating glycerol stocks.</td>
@@ Line 141: / Line 141: @@
 </tr>
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-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2821%29_.JPG | 21]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2821%29_.JPG”>21</a></td>
    <td>14/07/14</td>
    <td>GFP and RFP resuspension and transformation.</td>
@@ Line 147: / Line 147: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2822%29_.JPG | 22]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2822%29_.JPG”>22</a></td>
    <td>14/07/14</td>
    <td>GFP and RFP resuspension and transformation, cont.</td>
@@ Line 153: / Line 153: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2823%29_.JPG | 23]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2823%29_.JPG”>23</a></td>
    <td>16/07/14</td>
    <td>Mini-prepping GFP and RFP.</td>
@@ Line 159: / Line 159: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2824%29_.JPG | 24]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2824%29_.JPG”>24</a></td>
    <td>16/07/14</td>
    <td>GFP and RFP digestion/ligation to PSB1C3.</td>
@@ Line 165: / Line 165: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2825%29_.JPG | 25]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2825%29_.JPG”>25</a></td>
    <td>16/07/14</td>
    <td>Plasmid digestions.</td>
@@ Line 171: / Line 171: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2826%29_.JPG | 26]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2826%29_.JPG”>26</a></td>
    <td>16/07/14</td>
    <td>RFP/GFP ligations.</td>
@@ Line 177: / Line 177: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2827%29_.JPG | 27]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2827%29_.JPG”>27</a></td>
    <td>16/07/14</td>
    <td>RFP/GFP ligations, cont.</td>
@@ Line 183: / Line 183: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2828%29_.JPG | 28]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2828%29_.JPG”>28</a></td>
    <td>17/07/14</td>
    <td>Transformation of GFP/RFP with terminator.</td>
@@ Line 189: / Line 189: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2829%29_.JPG | 29]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2829%29_.JPG”>29</a></td>
    <td>18/07/14</td>
    <td>Making LB agar for promoters experiment.</td>
@@ Line 195: / Line 195: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2830%29_.JPG | 30]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2830%29_.JPG”>30</a></td>
    <td>18/07/14</td>
    <td>Promoter experiment – quantities.</td>
@@ Line 201: / Line 201: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2831%29_.JPG | 31]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2831%29_.JPG”>31</a></td>
    <td>18/07/14</td>
    <td>Promoter experiment – quantities, cont.</td>
@@ Line 207: / Line 207: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2832%29_.JPG | 32]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2832%29_.JPG”>32</a></td>
    <td>18/07/14</td>
    <td>Promoter experiment – quantities, cont. 2.</td>
@@ Line 213: / Line 213: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2833%29_.JPG | 33]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2833%29_.JPG”>33</a></td>
    <td>21/07/14</td>
    <td>Promoter experiment preliminary timetable.</td>
@@ Line 219: / Line 219: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2834%29_.JPG | 34]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2834%29_.JPG”>34</a></td>
    <td>22/07/14</td>
    <td>Electrophoresis of RFP and GFP (with terminators).</td>
@@ Line 225: / Line 225: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2835%29_.JPG | 35]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2835%29_.JPG”>35</a></td>
    <td>22/07/14</td>
    <td>Preparation of competent E. coli cells.</td>
@@ Line 231: / Line 231: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2836%29_.JPG | 36]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2836%29_.JPG”>36</a></td>
    <td>23/07/14</td>
    <td>GFP/RFP + terminator liquid broths mini-prepped.</td>
@@ Line 237: / Line 237: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2837%29_.JPG | 37]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2837%29_.JPG”>37</a></td>
    <td>23/07/14</td>
    <td>Potassium Chromate preparation.</td>
@@ Line 243: / Line 243: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2838%29_.JPG | 38]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2838%29_.JPG”>38</a></td>
    <td>23/07/14</td>
    <td>Transformation of other promoters.</td>
@@ Line 249: / Line 249: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2839%29_.JPG | 39]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2839%29_.JPG”>39</a></td>
    <td>24/07/14</td>
    <td>Moving GFP+T and RFP+T onto AMP backbones.</td>
@@ Line 255: / Line 255: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2840%29_.JPG | 40]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2840%29_.JPG”>40</a></td>
    <td>24/07/14</td>
    <td>Ligation of GFP+T and RFP+T onto AMP backbones.</td>
@@ Line 261: / Line 261: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2841%29_.JPG | 41]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2841%29_.JPG”>41</a></td>
    <td>24/07/14</td>
    <td>Potassium Dichromate colorimetry and spectrophotometry.</td>
@@ Line 267: / Line 267: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2842%29_.JPG | 42]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2842%29_.JPG”>42</a></td>
    <td>28/07/14</td>
    <td>Plating Anderson RBSs.</td>
@@ Line 273: / Line 273: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2843%29_.JPG | 43]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2843%29_.JPG”>43</a></td>
    <td>28/07/14</td>
    <td>Mini-prep of reporters, promoters and RBSs.</td>
@@ Line 279: / Line 279: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2844%29_.JPG | 44]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2844%29_.JPG”>44</a></td>
    <td>29/07/14</td>
    <td>COSHH Form created for Nitroglycerine experiments.</td>
@@ Line 285: / Line 285: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2845%29_.JPG | 45]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2845%29_.JPG”>45</a></td>
    <td>30/07/14</td>
    <td>Cr(VI) / Ligand experimentation.</td>
@@ Line 291: / Line 291: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2846%29_.JPG | 46]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2846%29_.JPG”>46</a></td>
    <td>31/07/14</td>
    <td>Mini-prep of constructs.</td>
@@ Line 297: / Line 297: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2847%29_.JPG | 47]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2847%29_.JPG”>47</a></td>
    <td>31/07/14</td>
    <td>Digestion and ligation of promoter/RBS combos.</td>
@@ Line 303: / Line 303: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2848%29_.JPG | 48]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2848%29_.JPG”>48</a></td>
    <td>31/07/14</td>
    <td>Oligo preparation.</td>
@@ Line 309: / Line 309: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2849%29_.JPG | 49]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2849%29_.JPG”>49</a></td>
    <td>31/07/14</td>
    <td>Ligation of promoter and RBs digestions.</td>
@@ Line 315: / Line 315: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2850%29_.JPG | 50]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2850%29_.JPG”>50</a></td>
    <td>01/08/14</td>
    <td>Digestion and Ligation of constructs 004 and 007.</td>
@@ Line 321: / Line 321: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2851%29_.JPG | 51]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2851%29_.JPG”>51</a></td>
    <td>01/08/14</td>
    <td>Digestion and Ligation of constructs 004 and 007, cont.</td>
@@ Line 327: / Line 327: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2852%29_.JPG | 52]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2852%29_.JPG”>52</a></td>
    <td>05/08/14</td>
    <td>Colonies picked and mini-prepped.</td>
@@ Line 333: / Line 333: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2853%29_.JPG | 53]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2853%29_.JPG”>53</a></td>
    <td>05/08/14</td>
    <td>Colonies picked and mini-prepped, cont.</td>
@@ Line 339: / Line 339: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2854%29_.JPG | 54]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2854%29_.JPG”>54</a></td>
    <td>06/08/14</td>
    <td>Testing promoter/RBS combination efficiency.</td>
@@ Line 345: / Line 345: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2855%29_.JPG | 55]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2855%29_.JPG”>55</a></td>
    <td>06/08/14</td>
    <td>Testing promoter/RBS combination efficiency, cont.</td>
@@ Line 351: / Line 351: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2856%29_.JPG | 56]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2856%29_.JPG”>56</a></td>
    <td>07/08/14</td>
    <td>Picking colonies from promoter/RBS combination transformations. </td>
@@ Line 357: / Line 357: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2857%29_.JPG | 57]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2857%29_.JPG”>57</a></td>
    <td>07/08/14</td>
    <td>T. Cam experiment.</td>
@@ Line 363: / Line 363: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2858%29_.JPG | 58]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2858%29_.JPG”>58</a></td>
    <td>11/08/14</td>
    <td>Promoter/RBS combinations again.</td>
@@ Line 369: / Line 369: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2859%29_.JPG | 59]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2859%29_.JPG”>59</a></td>
    <td>11/08/14</td>
    <td>Promoter/RBS combinations again, cont.</td>
@@ Line 375: / Line 375: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2860%29_.JPG | 60]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2860%29_.JPG”>60</a></td>
    <td>11/08/14</td>
    <td>Inoculation of enzymes for construct 001 and 003.</td>
@@ Line 381: / Line 381: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2861%29_.JPG | 61]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2861%29_.JPG”>61</a></td>
    <td>12/08/14</td>
    <td>Inoculation of enzymes for construct 001 and 003, cont.</td>
@@ Line 387: / Line 387: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2862%29_.JPG | 62]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2862%29_.JPG”>62</a></td>
    <td>12/08/14</td>
    <td>Transformation of a sample promoter/RBS combination.</td>
@@ Line 393: / Line 393: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2863%29_.JPG | 63]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2863%29_.JPG”>63</a></td>
    <td>12/08/14</td>
    <td>T. Cam experiment for solvents and ether.</td>
@@ Line 399: / Line 399: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2864%29_.JPG | 64]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2864%29_.JPG”>64</a></td>
    <td>13/08/14</td>
    <td>Combination transformation results and construct testing.</td>
@@ Line 405: / Line 405: @@
 </tr>
 <tr>
-   <td>[[media:Exeter_iGEM_2014_Lab_Book_Write-Up_%2865%29_.JPG | 65]]</td>
+   <td><a href=“Exeter_iGEM_2014_Lab_Book_Write-Up_%2865%29_.JPG”>65</a></td>
    <td>13/08/14</td>
    <td>Putting oligos into GFP and RFP.</td>

Team:Exeter/LabBook

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Revision as of 01:08, 18 October 2014

Lab Book