Difference between revisions of "Team:IIT Delhi/Notebook"

 
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     <div class="dropdown-content">
 
     <div class="dropdown-content">
 
       <a href="/Team:IIT_Delhi/Circuit_Design">Circuit design and construction</a>
 
       <a href="/Team:IIT_Delhi/Circuit_Design">Circuit design and construction</a>
       <a href="/Team:IIT_Delhi/Microfluidics">Microfluidics and Fluroscence</a>
+
       <a href="/Team:IIT_Delhi/Microfluidics">Microfluidics and Fluorescence</a>
 
       <a href="/Team:IIT_Delhi/Photobleaching">Photobleaching</a>
 
       <a href="/Team:IIT_Delhi/Photobleaching">Photobleaching</a>
 
       <a href="/Team:IIT_Delhi/Promoter">Promoter strength</a>
 
       <a href="/Team:IIT_Delhi/Promoter">Promoter strength</a>
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  <h2  class="boogaloo_font1 ">
 
  
20/4<br><ul>
 
<li>First team meet up
 
<li>Introduction of team members</ul><br>
 
25/4<br><ul>
 
<li> Discussion on DNA structure and replication, Chargaff’s rule, primers and enzymes</ul><br>
 
27/4<br><ul>
 
<li> Discussion on plasmids, digestion, ligation, transformation and 3A assembly
 
<li> Brainstorming on this year’s project - square wave generator</ul><br>
 
28/4<br><ul>
 
<li>Discussion on reference papers of repressilator, synchronous oscillations,
 
robustness etc.</ul><br>
 
29/4<br><ul>
 
<li> Discussion on Gel electrophoresis and blue-white screening</ul><br>
 
  
</h2>
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       <h2  class="boogaloo_font "><span style="font-size:30px;line-height:30px;cursor:pointer;display:block">We planned early on to document the work we did and efforts we put into our project, on a daily basis,hence, we were able to compile a comprehensive notebook accounting for all the events that took place.<br><br>April</span></h2>
  </div>
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  No probs... you can <a href="https://static.igem.org/mediawiki/2017/5/52/T--IIT_Delhi--NoteApril.pdf">click here to
 
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  download the PDF file.</a></p> 
       <h2  class="boogaloo_font "><span style="font-size:30px;cursor:pointer" onclick="openNav()">april</span></h2>
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To read...</p>
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01/05<br>
+
First lab visit of the team and instructions on how to handle the instruments and
+
safety guidelines were presented<br>
+
02/05<br>
+
<ol>
+
<li> Practicing inoculation, streaking and spreading of bacterial cultures of a biobrick used
+
in previous year
+
<li> LA plates and LB media preparation</ol><br>
+
03/05<br>
+
<ol>
+
<li> Practicing plasmid isolation and transformation with the part inoculated yesterday
+
<li> Inoculation of following parts from iGEM kit plate:-
+
<ul>
+
<li> RBS + GFP + T(without deg tag)
+
<li> RBS + TetR + T
+
<li>SYFP2
+
<li> J23119 promoter
+
<li> J23107 promoter</ul><br>
+
<li> Plasmid isolation of :-<br>
+
<ul>
+
<li> RBS + GFP + T(without deg tag)
+
<li> RBS + TetR + T
+
<li> SYFP2
+
<li> J23119 promoter
+
<li> J23107 promoter</ul><br>
+
<li> Transformation of plasmids mentioned previously following iGEM protocol</ol><br>
+
04/05<br>
+
<ol>
+
<li> Discussion on toggles switches and oscillators in relation to iGEM IITD project - 2016.
+
More detailed discussion on light activated self-repression and its effect on oscillator
+
frequency.
+
<li> Discussion on IITD 2015 project
+
<li> Discussion on some iGEM projects of other countries.
+
<li> Received the colonies transformed yesterday</ol><br>
+
06/05<br>
+
Further discussion on the research papers and different aspects of project<br>
+
09/05<br>
+
Formation of a marketing and human practices team and discussion on marketing
+
strategies used last year.<br>
+
11/05<br>
+
<ol>
+
<li>Video and content for crowd-funding initiative
+
<li>Mails and calls to potential sponsors</ol><br>
+
13/05<br>
+
<ol><li>Discussion on gene regulation in prokaryotes and eukaryotes with special emphasis on
+
prokaryotes.
+
<li> Discussion on how we can modify the Lac system by keeping its switching on properties
+
intact and replacing the gene part with, suppose, insulin such that presence Lactose
+
molecules trigger the activation of insulin gene.
+
<li> Discussion on the different class of promoters.</ol><br>
+
15/05<br>
+
<ol>
+
<li> Discussion on PCR
+
<li> Sample PCR product formed and ran on gel.</ol><br>
+
17/05
+
 1. Logic Gates:
+
a) AND GATE:
+
 
+
 discussion on simple AND gate
+
 AND gate with modified tRNA (Discussion on tRNA that would read TAG as Serine)
+
b) OR GATE
+
c) NOR GATE
+
d) XOR GATE: Using combination of different gates i.e. OR , AND , NOR, NAND, NOT and
+
further discussion on other ways of XOR gate formation.
+
 2. Steady state: Rate of accumulation=0
+
 3. Discussion on different equations for rate of change of protein and rate of change of RNA
+
(First and second order reactions) by discussing the journey from promoter to mRNA to
+
protein to nothingness.
+
 4. Enzyme Kinetics
+
 S+E === ES ----> P+E
+
 Differential equations of rate of change of ES and P discussed with equations of conservation
+
of mass for the same.
+
 Graphical analysis of ES/E0 vs S/S0 with discussion on quasi steady state.
+
 Graphical discussion on Concentration vs Time of the reaction.
+
 5. Michaelis menten equation
+
 6. Discussion on Degradation Tag and how it works in a bacterium where translation and
+
transcription happen in the same compartment and there are no stop codons.
+
 7. Discussion on Cancer Cell about how it was thought to find a cure of cancer using
+
these logic gates with inputs as miRNA(regulate genes) and output as apoptosis.
+
 8. Example of virus that can be used as vectors for human cells. e.g. Vaccinia virus
+
18/05
+
 Discussion on ways to generate different signal responses in bacterial gene regulatory
+
circuits
+
22/05
+
 Discussion on :-
+
1) Chemotactic response in bacteria
+
2) Temporal and spatial response in chemotaxis
+
3) Mechanism of chemotaxis in bacteria flagellum
+
4) Electrical model of chemotaxis
+
5) Adaptation time of chemotaxis
+
6) Finding electrical analogue of the biological system by varying frequency of the electrical circuit
+
made
+
7) Finding optimal frequency
+
8) Biological Robustness and causes of it in a biological system
+
9) System controls, bistability, modularity, buffering, bow-tie framework, decoupling
+
10) Robustness in signal transduction pathways and insect's segmental development
+
11) Robustness trade-offs
+
24/05
+
 Discussion on :-
+
1) Design principles of biochemical oscillators
+
2) Time delay's relevance in oscillation
+
3) Introduction of time delay with Intermediates
+
4) Limit cycles, conservative cycles and circadian rhythms
+
5) Time delay by positive feedback
+
6) Different classes of feedback
+
7) Linear and hyperbolic response
+
8) Goldbeter Kosher Function
+
9) Sniffers
+
10) Toggle Switch
+
 
+
11) Mutual inhibition and mutual activation
+
26/05
+
 Discussion on :-
+
1) A brief review of Sniffers, Buzzers and Toggle switch
+
2) Negative feedback oscillations
+
3) Positive feedback oscillations
+
4) Neutral feedback oscillations
+
5) Sub-critical and Super-critical hop bit
+
6) Study of mitosis
+
27/05
+
 Prepared lab supplies like LA, LB etc. to be used in the lab
+
29/05
+
1) Preparation of LuxI and PLux double digest using restriction enzymes EcoRI and PstI
+
2) Preparation of buffer and electrophoresis gel
+
3) Loading ladder, control and digest in the wells in gel
+
4) Electrophoresis and subsequent observation of gel to ensure digestion of plasmids
+
31/05
+
Discussion on:-
+
1) Plasmid isolation
+
2) Lysis solutions and their composition
+
3) Function of each component in the solutions
+
 
+
</h2>
+
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      <h2  class="boogaloo_font "><span style="font-size:30px;cursor:pointer" onclick="openNav()">May</span></h2>
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To read...</p>
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      <h2  class="boogaloo_font "><span style="font-size:30px;cursor:pointer">May</span></h2>
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    <div class="content1  boogaloo_font"><h2 class="boogaloo_font "><span style="font-size:30px;cursor:pointer" >July</span></h2>
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      <h2 class="boogaloo_font "><span style="font-size:30px;cursor:pointer" onclick="openNav()">july</span></h2>
 
 
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    <div class="content1  boogaloo_font"><h2 class="boogaloo_font "><span style="font-size:30px;cursor:pointer" >August</span></h2>
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Latest revision as of 22:19, 1 November 2017

iGEM IIT Delhi

We planned early on to document the work we did and efforts we put into our project, on a daily basis,hence, we were able to compile a comprehensive notebook accounting for all the events that took place.

April

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May

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June

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July

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August

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September

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October

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