Difference between revisions of "Team:Macquarie Australia/Notebook"

Revision as of 09:20, 14 October 2017

The first week involved learning all about synthetic biology and what lies ahead in terms of the competition
Dr Louise Brown and explained all things iGEM including the biobrick system and 3A assembly
An overview of the chlorophyll biosynthesis pathway, photosystem II and hydrogenase activity presented by Professor Robert Willows since our project would focus on one component of this bigger picture

Our project being to use biosynthetic techniques to create the hydrogen producing hydrogenase

We started planning for creation of complete hydrogenase plasmid by combining the Ferredoxin/Ferredoxin reductase biobrick with the Hyd1 biobrick

From this we expect some preliminary production of hydrogen however, with the addition of maturation enzymes this production would be maximised.

Discussion on construction of the maturation plasmid in which HydE/HydF biobrick would be combined with HydG biobrick then the two larger constructs would be ligated together to create the complete plasmid coding for the total Hydrogenase molecular machine, fondly named Omega Ω
We created a “3-day plan” from 3A assembly through transformation and plating up cells to liquid media overnight cultures, miniprep kit extraction of plasmid and nanodrop concentration measurement, and finally electrophoresis gel screening of our newly made construct
Discussion on human outreach was started.

Began talking to the SDU iGEM team on collaboration
Discussed the creation of an iGEM Macquarie game
Started planning for attending synthetic biology conference and ACUR (Adelaide).

India suggested the idea of a creating a game as her brother could help us out with that.
We got in contact with Joanne Jamie, an academic at Macquarie University, to gain more information about National Science Week and the university’s Orientation Day for our outreach possibilities.

She invited us to help out in the Chifley School Program (19th September) which we agreed would be better than the other two. We have a 1 hour time slot in which we can conduct wet and dry lab activities with gifted and talented high school science students.

Checked lab supplies to ensure we had what we needed.
Became familiar with protocols we will be using.
Poured LB plates made up with each of the three antibiotics we will be using- Amp, Kan and CAM.
Conducted three transformations of DHα5 cells with DNA plasmids of Fer, Hyd1 and HydEF.

Results = no growth on the plates.
This lead us to testing all our restriction enzymes on familiar plasmids, which gave us a chance to pour our own electrophoresis gel, load and run it.
It was great to have Mike Gibbs, Dominic Logel, Thi Huynh and Ed Moh supervising and sharing their expertise.

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+<tr>
+<td> <top> <img class="media object pull-left" src="https://static.igem.org/mediawiki/2017/8/81/T--Macquarie_Australia--flasklogo_.png" alt="flasklogo" style= "height:50%; width:50%">
+</td>
+<td>
+<h4> Wet Lab  </h4>
+<ul>
+<li> Checked lab supplies to ensure we had what we needed. </li>
+<li> Became familiar with protocols we will be using. </li>
+<li> Poured LB plates made up with each of the three antibiotics we will be using- Amp, Kan and CAM. </li>
+<li> Conducted three transformations of DHα5 cells with DNA plasmids of Fer, Hyd1 and HydEF. </li>
+<ul>
+<li> These were grown successfully on plates. </li>
+</ul>
+<li> Dived into our first ligation attempt for Fer/Hyd following our “3-day plan” </li>
+<ul>
+<li> Results = no growth on the plates.</li>
+<li> This lead us to testing all our restriction enzymes on familiar plasmids, which gave us a chance to pour our own electrophoresis gel, load and run it. </li>
+<li> It was great to have Mike Gibbs, Dominic Logel, Thi Huynh and Ed Moh supervising and sharing their expertise.</li>
+</ul>
+</td>
+</tr>
+</table>
+</p>
+</div>
+</body>
+</div>