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

Revision as of 15:27, 12 September 2015

Sept 17

First meeting of Team:IIT_Madras for iGEM 2015.
Ideation begins.

May 18-24

May 25-31

Inventory of all supplies is to be done.
Alyteserin-1a was chosen to test our model as the structural feature, mechanism of action and other relevent details of anit-microbial peptide Alyteserin-1c, which has two mutations (D4E, N23S), were available in the literature.
The pdb structure of Alyteserin-1a was generated in pymol, while introducing two mutations D4E and S23N in the pdb structure of Alyteserin-1c.
The structural features of Alyteserin-1a was analyzed carefully to design a novel peptide which could interact with it.
Pymol and Pepstr, an online tool, were used to generate a large number of peptide pdb structures of size 10-18 amino acid.
A software, ZDOCK, was used to assess the docking parameters of Alyteserin-1a and novel peptide.
Best peforming peptide was chosen to test it's functionality in molecular dynamic simulation.

June 1-7

Molecul Dynamic Simulation started.
Made a catalog of all available materials.
Lacto Bacilus strains, NZ9000 and MG1363, were collected from Prof. KBR's lab.
MD Simulations finished the proteins were found to interact favourably.

June 8-14

Started working on the design of genetic circuit.
One more MD Simulation was performed with the ionic solution of protein complex. MD Simultions showed that naly interacts favorably with Alyteserin forming a cavity of hydrophobic residues.
Sender is finalised to be E.Coli DH5Alpha with LuxP-PFS gene.
Receiver is L.lactis NZ9000/MG1316 with LUXPQOU coupled with Lux R through sRNA's qrr1-5, HFQ and sigma54 gene.

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@@ Line 1: / Line 1: @@
 {{IIT_Madras}}
 <html>
+<h2>Sept 17</h2>
+<ul>
+<li>First meeting of Team:IIT_Madras for iGEM 2015.</li>
+<li>Ideation begins.</li>
+</ul>
 <h2>May 18-24</h2>
 <ul>
-<li>Cleaned fridge and transferred materials.</li>
+<li></li>
-<li>Circuit finalised toggle switch/ mutual depressor switch using TAL repressor.</li>
+<li></li>
 </ul>
@@ Line 23: / Line 31: @@
-<h3> June 1-7</h3>
+<h3>June 1-7</h3>
 <ul>
-<li> MoleculGROMACS simulations started
+<li>Molecul Dynamic Simulation started.</li>
--> Made a catalog of all available materials
+<li>Made a catalog of all available materials.</li>
--> Lacto Bacilus strains are available NZ9000 and MG1363
+<li>Lacto Bacilus strains, NZ9000 and MG1363, were collected from Prof. KBR's lab.</li>
--> Simulations finished the proteins were found to interact favourably
+<li>MD Simulations finished the proteins were found to interact favourably.</li>
--> Heidelberg 2008 Auto Inducer 2 produced by LuxS sensed by LuxQ
+</ul>
--> Reference:Quorum Sensing AI@ in campylobacter Orla Cloak, Barbara Solow doi:10.1128
-Can we do the whole circuit using just Lux components??!!
---------------------------------------------------------
-Week 4
+<h3>June 8-14</h3>
+<ul>
-->Circuit will be composed of purely Lux components.
+<li>Started working on the design of genetic circuit.</li>
--> MD Simulations were done with ionic solution of protein complex. MD Simultions showed that naly
+<li>One more MD Simulation was performed with the ionic solution of protein complex. MD Simultions showed that naly
-interacts favorably with Alytesterin forming a cavity of hydrophobic residues
+interacts favorably with Alyteserin forming a cavity of hydrophobic residues.</li>
--> Sender is finalised to be E.Coli DH5Alpha with LuxP-PFS gene
+<li>Sender is finalised to be E.Coli DH5Alpha with LuxP-PFS gene.</li>
-Receiver is L.lactis NZ9000/MG1316 with LUXPQOU coupled with Lux R through sRNA's qrr1-5 and HFQ
+<li>Receiver is L.lactis NZ9000/MG1316 with LUXPQOU coupled with Lux R through sRNA's qrr1-5, HFQ and sigma54 gene.</li>
+</ul>
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