Template:Team:SydneyUni Australia/Calendar/Events List

From 2013.igem.org

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events: [
events: [
-
// -----------------Early days ----------------
+
// -----------------Early days ----------------
-
{
+
{ title: 'First Meeting',
-
title: 'First Meeting',
+
start: new Date(2012, 12, 31),
-
start: new Date(2012, 12, 31),
+
description: 'Coleman, Rob<br>Robbie introduces iGEM to potential supervisors around campus. Coleman pricks his ears. '
-
description: '<b>Members:</b> Coleman, Rob <br> <b>What we did: </b> Robbie introduces iGEM to potential supervisors around campus. Coleman pricks his ears. '
+
},
-
},
+
{ title: 'Advisor Meeting',
-
// -----------------Early days 2 ----------------
+
start: new Date(2013, 2, 14),
-
{
+
description: 'Rob<br>Robbie introduces iGEM to the Manager of Inspiring Australia in NSW, facilitator for National Science Week. Advice '},
-
title: 'Advisor Meeting',
+
{ title: 'First Team Meeting',
-
start: new Date(2013, 2, 14),
+
start: new Date(2013, 2, 18),
-
description: '<b>Members:</b> Rob <br> <b>What we did: </b>Robbie introduces iGEM to the Manager of Inspiring Australia in NSW, facilitator for National Science Week. Advice '
+
description: 'Rob, Andrew, Viv, Shuravi, Cyril, Desmond, Hugh, Evelyn<br>First team meeting at Hermann’s. We talked about some crazy outreach ideas like gfp graffiti and organizing a symposium. The seed that became Strange Nature was planted. A lot of support for DCA degradation and Botany Bay as our lab project. '},
-
},
+
{ title: 'CLC meeting',
-
// -----------------Early days 3 ----------------
+
start: new Date(2013, 2, 26),
-
{
+
description: 'Rob, Andrew<br>Attend the CLC Town Hall Meeting held by Orica at Botany Bay. We introduce iGEM and our project and look for possible collaborators. ' },
-
title: 'First Team Meeting',
+
{ title: 'Project planning',
-
start: new Date(2013, 2, 18),
+
start: new Date(2013, 3, 9),
-
description: '<b>Members:</b> Rob, Andrew, Viv, Shuravi, Cyril, Desmond, Hugh, Evelyn <br> <b>What we did: </b>First team meeting at Hermann’s. We talked about some crazy outreach ideas like gfp graffiti and organizing a symposium. The seed that became Strange Nature was planted. A lot of support for DCA degradation and Botany Bay as our lab project.  
+
description: 'Nick, Rob, Andrew, Viv, Shuravi, Cyril, Desmond, Hugh, Evelyn<br>Learned that we won’t be able to use Mox from Xanthobacter autotrophicus as planned due to the reliance on co-factor PQQ. Began considering a monooxygenase pathway for degradation. ' },
-
},
+
{ title: 'Meeting Yagiz',
-
// -----------------Early days 4 ----------------
+
start: new Date(2013, 4, 3),
-
{
+
description: 'Nick, Rob, Andrew, Viv, Shuravi, Cyril, Desmond, Hugh, Evelyn<br>Met with Yagiz and Rob from the MQ University iGEM team for a general introduction to iGEM and some helpful advice.'},
-
title: 'CLC meeting',
+
{ title: 'Tutorial on primer design. ',
-
start: new Date(2013, 2, 26),
+
start: new Date(2013, 4, 14),
-
description: '<b>Members:</b> Rob, Andrew<br> <b>What we did: </b>Attend the CLC Town Hall Meeting held by Orica at Botany Bay. We introduce iGEM and our project and look for possible collaborators.
+
description: 'Nick, Rob, Andrew, Viv, Shuravi, Cyril, Desmond, Hugh, Evelyn<br>Tutorial on primer design for designing primers for the project'},
-
},
+
// -----------------Week 1 ----------------
-
// -----------------Early days 5 ----------------
+
{ title: 'Lab Setup',
-
{
+
start: new Date(2013, 4, 17),
-
title: 'Project planning',
+
description: 'Coleman, Viv, Desmond, Rob and Hugh<br>We made some solutions of LB, LB agar and TE. We staked out our claim in the lab. Yay!'},
-
start: new Date(2013, 3, 9),
+
{ title: 'ToMO plasmid Extraction',
-
description: '<b>Members:</b> Nick, Rob, Andrew, Viv, Shuravi, Cyril, Desmond, Hugh, Evelyn<br> <b>What we did: </b>Learned that we won’t be able to use Mox from Xanthobacter autotrophicus as planned due to the reliance on co-factor PQQ. Began considering a monooxygenase pathway for degradation.  
+
start: new Date(2013, 4, 22),
-
},
+
description: 'Coleman, Andrew, Desmond and Shuravi<br>We started the plasmid extraction of ToMO from the E. coli.'},
-
// -----------------Early days 6 ----------------
+
{ title: 'ToMO plasmid Extraction',
-
{
+
start: new Date(2013, 4, 23),
-
title: 'Meeting Yagiz',
+
description: 'Coleman, Andrew, Cyril<br>Continued the ToMO plasmid prep. Reached the step where DNA is precipitated in ethanol and acetate overnight'},
-
start: new Date(2013, 4, 3),
+
{ title: 'ToMO plasmid Extraction',
-
description: '<b>Members:</b> Nick, Rob, Andrew, Viv, Shuravi, Cyril, Desmond, Hugh, Evelyn<br> <b>What we did: </b>Met with Yagiz and Rob from the MQ univeristy iGEM team for a general introduction to iGEM and some helpful advice.  
+
start: new Date(2013, 4, 24),
-
},
+
description: 'Coleman, Viv, Rob<br>Finished the ToMO plasmid prep. Digested pBBR1-MCS2. Used the nanodrop. Did a digest + gel of our ToMO, undigested and Xbal1-digested pBBR along with a marker'},
-
// -----------------Early days 7 ----------------
+
// -----------------Week 2 ----------------
-
{
+
{ title: 'Transformation and Selection',
-
title: 'Tutorial on primer design. ',
+
start: new Date(2013, 4, 29),
-
start: new Date(2013, 4, 14),
+
description: 'Coleman, Cyril, Shuravi, Rob<br>We transformed E. coli Epi300 with two plasmids, pBBR and pBS(ToMO). As both have Km resistance, only those cells that were successfully transformed with the plasmid would grown when plated onto LB+Km media. They were incubated overnight'},
-
description: '<b>Members:</b> Nick, Rob, Andrew, Viv, Shuravi, Cyril, Desmond, Hugh, Evelyn<br> <b>What we did: </b>Tutorial on primer design for designing primers for the project
+
{ title: 'Intro to Gibson',
-
},
+
start: new Date(2013, 4, 29),
-
// -----------------Week 1 ----------------
+
description: 'Nick, Cyril, Andrew, Rob<br>We discussed Gibson Assembly and gBlocks for the first time, due to concerns about having enough time.'},
-
{
+
{ title: 'Growing up cells',
-
title: 'Lab Setup',
+
start: new Date(2013, 4, 30),
-
start: new Date(2013, 4, 17),
+
description: 'Coleman, Andrew, Desmond<br>The two E. Coli treatments were growing at different rates, E. Coli (pBS-ToMO) wasn’t growing well at all. We transferred E. Coli (pBBR) to broth and later washed and transferred to two phosphate buffer treatments, one with DCA, one without. We transferred E. Coli (pBS-ToMO) to broth and incubated it overnight. DCA concentration was 1mM. '},
-
description: '<b>Members:</b> Coleman, Viv, Desmond, Rob and Hugh <br> <b>What we did: </b> We made some solutions of LB, LB agar and TE. We staked out our claim in the lab. Yay!'
+
{ title: 'Chloride Assay',
-
},
+
start: new Date(2013, 4, 31),
-
{
+
description: 'Coleman, Rob, Hugh<br>After 24 hours in DCA, we put E. Coli (pBBR) in the cool room for a Cl assay next week. We washed and transferred E. Coli (pBS-ToMO) from broth to two phosphate buffer treatments, one with DCA, one without. We also ran a quick PCR testing our new ToMO primers on pBS-ToMO, but we didn’t digest pBS-ToMO before PCR. !'},
-
title: 'ToMO plasmid Extraction',
+
// -----------------Week 3 ----------------
-
start: new Date(2013, 4, 22),
+
{ title: 'Meeting with Yagiz',
-
description: '<b>Members:</b> Coleman, Andrew, Desmond and Shuravi <br> <b>What we did: </b> We started the plasmid extraction of ToMO from the E. coli.'
+
start: new Date(2013, 5, 2),
-
},
+
description: 'Rob<br>We met with Yagiz at Macquarie University to talk about Strange Nature and possible collaboration with our iGEM teams.'},
-
{
+
{ title: 'PCR analysis and GC analysis of DCA metabolism',
-
title: 'ToMO plasmid Extraction',
+
start: new Date(2013, 5, 3),
-
start: new Date(2013, 4, 23),
+
description: 'Coleman, Hugh, Rob<br>We ran a gel of last Friday’s PCR. The PCR was of pBS(ToMO) extracted from Wood’s E. Coli TG1, with primers iGEM 1 & 2. The banding on the gel was obscure, potentially due to too much template and could not be used.<br><br>We used the Gas Chromatographer (GC) to look at our two DCA treatments of E. Coli (transformed with either pBBR or pBS(ToMO)). Both had pretty much the same reading but it is uncertain yet whether this is because pBS(ToMO) was lost or altered during the extended incubation from Week 2, or whether ToMO was unable to degrade DCA. We also set up standardised solutions of NaCl in KP buffer for a future Cl assay.'},
-
description: '<b>Members:</b> Coleman, Andrew, Cyril <br> <b>What we did: </b> Continued the ToMO plasmid prep. Reached the step where DNA is precipitated in ethanol and acetate overnight'
+
// -----------------Week 4 ----------------
-
},
+
 
-
{
+
{ title: 'Redo of ToMO Trial',
-
title: 'ToMO plasmid Extraction',
+
start: new Date(2013, 5, 22),
-
start: new Date(2013, 4, 24),
+
end: new Date(2013, 5, 27),
-
description: '<b>Members:</b> Coleman, Viv, Rob <br> <b>What we did: </b> Finished the ToMO plasmid prep. Digested pBBR1-MCS2. Used the nanodrop. Did a digest + gel of our ToMO, undigested and Xbal1-digested pBBR along with a marker'
+
description: 'Coleman, Rob<br>We repeated the ToMO trial however made some changes to the protocol.'},
-
},
+
// -----------------Week 5 ----------------
-
// -----------------Week 2 ----------------
+
{ title: 'Meeting Mac Uni Team',
-
{
+
start: new Date(2013, 6, 1),
-
title: 'Transformation and Selection',
+
description: 'Rob, Andrew, Viv, Shuravi, Desmond, Cyril<br>Lasertag and bowling with the Macquarie University iGEM team.'},
-
start: new Date(2013, 4, 29),
+
{ title: 'ToMO Chloride Assay',
-
description: '<b>Members:</b> Coleman, Cyril, Shuravi, Rob <br> <b>What we did: </b> We transformed E. coli Epi300 with two plasmids, pBBR and pBS(ToMO). As both have Km resistance, only those cells that were successfully transformed with the plasmid would grown when plated onto LB+Km media. They were incubated overnight'
+
start: new Date(2013, 6, 4),
-
},
+
description: 'Coleman, Cyril, Desmond, Shuravi<br>Performed chloride assay on ToMO, pBBR, TOM/+-DCA samples. ToMO came 1st place, with reasonable amounts of DCA metabolised.'},
-
{
+
// -----------------Week 6 ----------------
-
title: 'Intro to Gibson',
+
{ title: 'PCR of pBBR-mcs2 Origin',
-
start: new Date(2013, 4, 29),
+
start: new Date(2013, 6, 11),
-
description: '<b>Members:</b> Nick, Cyril, Andrew, Rob <br> <b>What we did: </b>We discussed Gibson Assembly and gBlocks for the first time, due to concerns about having enough time. '
+
end: new Date(2013, 6, 12),
-
},
+
description: 'Elissa, Cyril, Desmond, Rob<br>We tried to PCR the origin of replication from pBBR1-MCS2 using primer iGEM 5 and 6. We digested the plasmid with EcoR1 ran a diagnostic PCR but didn’t see anything. We re-digested the plasmid with a higher concentration of DNA, and did a gradient PCR, and didn’t see the desired PCR product. We’re looking into mispriming elsewhere on pBBR.'},
-
{
+
{ title: 'Gibson Planning',
-
title: 'Growing up cells',
+
start: new Date(2013, 6, 12),
-
start: new Date(2013, 4, 30),
+
description: 'Nick, Rob, Andrew, Viv, Shuravi, Desmond, Evelyn<br>Met to dicuss Gibson Assembly and decided to pursue this method of assembly. Delegated some tasks for finding sequences, optimisation and ordering of gBlocks from IDT using the special iGEM discount.'},
-
description: '<b>Members:</b> Coleman, Andrew, Desmond <br> <b>What we did: </b> The two E. Coli treatments were growing at different rates, E. Coli (pBS-ToMO) wasn’t growing well at all. We transferred E. Coli (pBBR) to broth and later washed and transferred to two phosphate buffer treatments, one with DCA, one without. We transferred E. Coli (pBS-ToMO) to broth and incubated it overnight. DCA concentration was 1mM. '
+
// -----------------Week 7 ----------------
-
},
+
{ title: 'Making competent PstQ',
-
{
+
start: new Date(2013, 6, 23),
-
title: 'Chloride Assay',
+
end: new Date(2013, 6, 24),
-
start: new Date(2013, 4, 31),
+
description: 'Desmond, Rob<br>We made competent PstQ for electroporation (Pseudomonas stutzeri, strain Q, the ones that are naturally competent for transformation, but we will also be testing our genes as plasmids).'},
-
description: '<b>Members:</b> Colman, Rob, Hugh<br> <b>What we did: </b> After 24 hours in DCA, we put E. Coli (pBBR) in the cool room for a Cl assay next week. We washed and transferred E. Coli (pBS-ToMO) from broth to two phosphate buffer treatments, one with DCA, one without. We also ran a quick PCR testing our new ToMO primers on pBS-ToMO, but we didn’t digest pBS-ToMO before PCR. !'
+
{ title: 'General Lab Stuff',
-
},
+
start: new Date(2013, 6, 26),
-
// -----------------Week 3 ----------------
+
description: 'Shuravi, Rob<br>Prepared for arrival of gBlocks by making up reagents for plasmid prep, pouring chloramphenicol. We also tested whether the prepared PstQ cells were competent and uncontaminated'},
-
+
// -----------------Week 8 ----------------
-
{
+
{ title: 'Gibson Assembly',
-
title: 'PCR analysis and GC analysis of DCA metabolism',
+
start: new Date(2013, 7, 12),
-
start: new Date(2013, 4, 3),
+
description: 'Andrew, Rob<br>gBlocks arrived at the end of last week. We did a Gibson Assembly reaction, and transformed the product into E. Coli (EPI300). These were incubated overnight.'},
-
description: '<b>Members:</b> Coleman, Hugh, Rob <br> <b>What we did: </b> We ran a gel of last Friday’s PCR. The PCR was of pBS(ToMO) extracted from Wood’s E. Coli TG1, with primers iGEM 1 & 2. The banding on the gel was obscure, potentially due to too much template and could not be used. <br><br> We used the Gas Chromatographer (GC) to look at our two DCA treatments of E. Coli (transformed with either pBBR or pBS(ToMO)). Both had pretty much the same reading but it is uncertain yet whether this is because pBS(ToMO) was lost or altered during the extended incubation from Week 2, or whether ToMO was unable to degrade DCA. We also set up standardised solutions of NaCl in KP buffer for a future Cl assay.'
+
{ title: 'Checking Gibson',
-
},
+
start: new Date(2013, 7, 13),
-
// -----------------Week 4 ----------------
+
description: 'Rob, Hugh<br>- The following morning (13th), nothing had grown. Our positive control showed that the transformation was successful, negative control that our technique was sterile.<br><br>- Ran a gel of pSB1C3 (the plasmid that the gBlocks are being assembled into), to confirm that we were sent a clean sample by the iGEM HQ.<br><br>- The Gibson Assembly was run again with only a positive control (a pUC19 plasmid with 5 gBlocks, provided by IDT), transformed and incubated overnight. The following morning  (14th) a few, small colonies were growing on ampicillin plates, indicating the pUC19 positive control has assembled correctly.' },
-
+
{ title: 'Gibson Assembly Take 2',
-
{
+
start: new Date(2013, 7, 14),
-
title: 'Redo of ToMO Trial',
+
end: new Date(2013, 7, 15),
-
start: new Date(2013, 5, 22),
+
description: 'Rob, Hugh, Shuravi, Desmond<br>A few different things were tried including:<br><br>- Transforming into a different E. Coli host (TOP10), since perhaps our home-made cells weren’t up to IDT’s standards.<br><br>- Transforming into the same host (EPI300) but letting the cells recover and incubate at room temperature. Perhaps our pathway assembled correctly but overexpression of foreign enzymes impeded cells at maximum growth rate. Results were the same as the original Gibson Assembly transformation.'},
-
end: new Date(2013, 5, 27),
+
// -----------------Week 9 ----------------
-
description: '<b>Members:</b> Coleman, Rob <br> <b>What we did: </b> We repeated the ToMO trial however made some changes to the protocol. '
+
{ title: 'Colony Screening',
-
},
+
start: new Date(2013, 7, 16),
-
// -----------------Week 5 ----------------
+
end: new Date(2013, 7, 18),
-
{
+
description: 'Rob, Nick, Desmond, Andrew<br>- Checked plates and learned that transforming our Gibson Assembly product into TOP10 (rather than EPI300) worked better than before.<br><br>- This was confirmed on Saturday morning (17th) after re-transforming the same reaction with the last of our Gibson Assembly product, in order to obtain more colonies for screening (for finding which of the colonies contains the correctly assembled pathway).<br><br>- A master plate containing all colonies was patched for phenotypic screening the following week.'},
-
title: 'ToMO Chloride Assay',
+
{ title: 'Chloride Assay',
-
start: new Date(2013, 6, 4),
+
start: new Date(2013, 7, 19),
-
description: '<b>Members:</b> Coleman, Cyril, Desmond, Shuravi<br> <b>What we did: </b> Performed chloride assay on ToMO, pBBR, TOM/+-DCA samples. ToMO came 1st place, with reasonable amounts of DCA metabolised. '
+
description: 'Rob, Vivian<br>Set-up 87 clones to incubate in chloroacetate overnight to detect Cl- release, indicating the presence of dhlB in pSB1C3.'},
-
},
+
{ title: 'Chloride Assay',
-
// -----------------Week 6 ----------------
+
start: new Date(2013, 7, 20),
-
{
+
description: 'Rob, Andrew, Desmond<br>[Cl-] assay of the 87 clones<br><br>Chose 10 of the clones based on the results (5 representing each pathway) and set-up broths for a plasmid prep and a second [Cl-] assay (taking cells from plates instead of broth).'},
-
title: 'PCR of pBBR-mcs2 Origin',
+
{ title: 'Chloride Assay, Plasmid Prep',
-
start: new Date(2013, 6, 9),
+
start: new Date(2013, 7, 21),
-
description: '<b>Members:</b> Rob, Elissa<br> <b>What we did: </b> I have no idea '
+
description: 'Rob, Shuravi, Hugh<br>[Cl-] assayed the 10 clones. Plasmid prepped the 10 clones.'},
-
},
+
{ title: 'Gel of Plasmid Prep',
-
{
+
start: new Date(2013, 7, 22),
-
title: 'PCR of pBBR-mcs2 Origin',
+
description: 'Rob, Nick<br>Ran a gel of yesterday’s plasmid prep and found it was too diluted and full of RNA.'},
-
start: new Date(2013, 6, 11),
+
{ title: 'Plasmid Prep Take 2',
-
end: new Date(2013, 6, 12),
+
start: new Date(2013, 7, 23),
-
description: '<b>Members:</b> Elissa, Cyril, Desmond, Rob<br> <b>What we did: </b> We tried to PCR the origin of replication from pBBR1-MCS2 using primer iGEM 5 and 6. We digested the plasmid with EcoR1 ran a diagnostic PCR but didn’t see anything. We re-digested the plasmid with a higher concentration of DNA, and did a gradient PCR, and didn’t see the desired PCR product. We’re looking into mispriming elsewhere on pBBR. '
+
description: 'Viv<br>Treated plasmids with RNAse, repeated final steps of plasmid prep.'},
-
},
+
// -----------------Week 10 ----------------
-
// -----------------Week 7 ----------------
+
{ title: 'Chloride Assay Prep',
-
{
+
start: new Date(2013, 7, 24),
-
title: 'Making competent PstQ',
+
end: new Date(2013, 7, 25),
-
start: new Date(2013, 6, 23),
+
description: 'Andrew, Nick<br>- Plated out cells carrying pUC19-dhlB for positive control in [Cl-] assay.<br><br>- Inoculated 4ml broths for [Cl-] assay'},
-
end: new Date(2013, 6, 24),
+
{ title: 'Chloride Assay',
-
description: '<b>Members:</b> Desmond, Rob<br> <b>What we did: </b> We made competent PstQ for electroporation (Pseudomonas stutzeri, strain Q, the ones that are naturally competent for transformation, but we will also be testing our genes as plasmids).'
+
start: new Date(2013, 7, 26),
-
},
+
description: 'Desmond<br>- Transferred overnight cultures (4mL) to fresh 50 mL LB and grown to an OD of ~1.0. Cells were harvested, cleaned and resuspended in 2mM chloroacetate for overnight incubation for chloride assay the next day.'},
-
{
+
{ title: 'Chloride Assay Stuff',
-
title: 'General Lab Stuff',
+
start: new Date(2013, 7, 27),
-
start: new Date(2013, 6, 26),
+
description: 'Rob<br>Remaining E.coli was spread plated onto Mackonkey agar for future negative Cl- assays.<br><br>Solutions for plasmid preps and chloride assays were made. We suspect the ambiguous plasmid prep and chloride assays results are due to poor stocks.'},
-
description: '<b>Members:</b> Shuravi, Rob<br> <b>What we did: </b> Prepared for arrival of gBlocks by making up reagents for plasmid prep, pouring chloramphenicol. We also tested whether the prepared PstQ cells were competent and uncontaminated '
+
{ title: 'Chloride Assay',
-
},
+
start: new Date(2013, 7, 28),
-
// -----------------Week 8 ----------------
+
description: 'Rob<br>Inoculated LB-Cm with our clones [2,10,38, 42,54,64, rfp(63)], LB-Am (positive control) and LB (negative control) for plasmid prep and chloride assay. No growth was observed in positive and negative control so no culture could be transferred for chloride assay.'},
-
{
+
{ title: 'Chloride Assay Stuff',
-
title: 'Gibson Assembly',
+
start: new Date(2013, 7, 29),
-
start: new Date(2013, 7, 12),
+
description: 'Rob, Shuravi, Desmond<br>Clones grown in LB-antibiotic broth overnight were washed and added to 2mM DCA reagents and another set in 2mM chloroacetate reagent.  Standards using NaCl solution was made simultaneously to ensure accuracy of the assay.<br><br>Plasmid preps were done using clones 2, 10, 38, 54, 42, 64 and rfp 63.<br><br>The samples were patch plated onto new LB-Cm plates.'},
-
description: '<b>Members:</b> Andrew, Rob<br> <b>What we did: </b> gBlocks arrived at the end of last week. We did a Gibson Assembly reaction, and transformed the product into E. Coli (EPI300). These were incubated overnight.'
+
// -----------------Week 11 ----------------
-
},
+
{ title: 'Diagnostic Gel',
-
{
+
start: new Date(2013, 7, 31),
-
title: 'Checking Gibson',
+
description: 'Rob<br>A diagnostic digest was set up for clones 42, 54 and 64 using EcoRV and 2, 38, rfp using EcrIVHF. Banding patterns on our gel was difficult to see but was better visualised under UV.'},
-
start: new Date(2013, 7, 13),
+
{ title: 'PCR Work',
-
description: '<b>Members:</b> Rob, Hugh<br> <b>What we did: </b> - The following morning (13th), nothing had grown. Our positive control showed that the transformation was successful, negative control that our technique was sterile. <br><br>- Ran a gel of pSB1C3 (the plasmid that the gBlocks are being assembled into), to confirm that we were sent a clean sample by the iGEM HQ. <br><br>- The Gibson Assembly was run again with only a positive control (a pUC19 plasmid with 5 gBlocks, provided by IDT), transformed and incubated overnight. The following morning  (14th) a few, small colonies were growing on ampicillin plates, indicating the pUC19 positive control has assembled correctly.'  
+
start: new Date(2013, 8, 2),
-
},
+
description: 'Rob, James<br>Our new primers arrived. Today we PCR screened for dhlB and found the reverse primer corresponded to the synthetic dhlB sequence. Our PCR products were then loaded onto gel. The results were a little disappointing as there was no banding on our first gel and the ladder was difficult to see. Primer dimers were observed on our gel.<br><br>We also inoculated another 20 clones for screening from our initial Gibson Assembly transformation of p-p [contains p450] and p-a [contains adh] (These are our two different pathways).<br><br>We prepared some competent EPI400 cells. These are to be used later for the transformation of our GA products.'},
-
{
+
{ title: 'Cell Transformation, Gibson Assembly',
-
title: 'Gibson Assembly Take 2',
+
start: new Date(2013, 8, 3),
-
start: new Date(2013, 7, 14),
+
description: 'Andrew, Rob<br>We transformed our Epi400 cells with our Gibson assembly products. Results did not look very promising. The Epi400 cells looked as they did when we transformed Epi300. The control worked and few cells grew with the positive Gibson assembly. There was more growth of cells transformed with p-p and p-a.<br><br>Another Gibson Assembly was set up for transformation. We found iGEMblock1 did not contain enough DNA leaving less than needed for the p-a sample.<br><br>We PCR screened for dhlB in colonies 100-139 however did not have a positive control (did not work yesterday). A gel was run for the dhlB PCR products.'},
-
end: new Date(2013, 7, 15),
+
{ title: 'Cell Transformation',
-
description: '<b>Members:</b> Rob, Hugh, Shuravi, Desmond<br> <b>What we did: </b> A few different things were tried including:<br><br>- Transforming into a different E. Coli host (TOP10), since perhaps our home-made cells weren’t up to IDT’s standards.<br><br>- Transforming into the same host (EPI300) but letting the cells recover and incubate at room temperature. Perhaps our pathway assembled correctly but overexpression of foreign enzymes impeded cells at maximum growth rate. Results were the same as the original Gibson Assembly transformation.'  
+
start: new Date(2013, 8, 4),
-
},
+
description: 'Rob<br>Another transformation was performed using the second set of Gibson assembly products into E.coli TOP 10 and E.coli Epi400.  The transformed cells were plated onto the appropriate antibiotic media.'},
-
// -----------------Week 9 ----------------
+
{ title: 'PCR and Diagnostic Gel',
-
{
+
start: new Date(2013, 8, 5),
-
title: 'Colony Screening',
+
description: 'Andrew<br>We did a PCR of dhlB from the GA reaction products using three samples (p-p, p-a and a negative control containing no DNA)<br><br>All GA enzymes were heat-killed by placing using thermocycler at 95 degrees.<br><br>We ran a gel of dhlB PCR of Gibson assembly products. The resulting bands were clear and as expected.'},
-
start: new Date(2013, 7, 16),
+
{ title: 'Diagnostic Gel',
-
end: new Date(2013, 7, 18),
+
start: new Date(2013, 8, 6),
-
description: '<b>Members:</b> Rob, Nick, Desmond, Andrew<br> <b>What we did: </b> - Checked plates and learned that transforming our Gibson Assembly product into TOP10 (rather than EPI300) worked better than before.<br><br>- This was confirmed on Saturday morning (17th) after re-transforming the same reaction with the last of our Gibson Assembly product, in order to obtain more colonies for screening (for finding which of the colonies contains the correctly assembled pathway).<br><br>- A master plate containing all colonies was patched for phenotypic screening the following week.'
+
description: 'Rob<br>A diagnostic digest was performed on our old plasmid preps. p-p was digested with BamH1, MluI, SmaI, SphI and Sal1. P-a digested with MluI, SmaI, SphI and rfp had no restriction enzyme added'},
-
},
+
// -----------------Week 12 ----------------
-
{
+
{ title: 'Digests',
-
title: 'Chloride Assay',
+
start: new Date(2013, 8, 9),
-
start: new Date(2013, 7, 19),
+
description: 'Andrew, Desmond, Rob<br>Two digests were set up in parallel (p-p and p-a) using SspI and later purified using Quiaquick columns.'},
-
description: '<b>Members:</b> Rob, Vivian<br> <b>What we did: </b>Set-up 87 clones to incubate in chloroacetate overnight to detect Cl- release, indicating the presence of dhlB in pSB1C3. '
+
{ title: 'Plasmid Prep, PCR Screen',
-
},{
+
start: new Date(2013, 8, 10),
-
title: 'Chloride Assay',
+
description: 'Andrew<br>A plasmid prep was performed on pSB-RFP, taken from transformed E.coli TOP10 cells. Stopped at precipitation stage.<br><br>We received our new set of primers! We used these to PCR screen all our selected Gibson assembly plasmids and GA restriction products and our positive GA control (puc19-dhlA-dhlB)<br><br>To confirm that our PCR screening had worked we ran a gel of all our PCR products'},
-
start: new Date(2013, 7, 20),
+
{ title: 'Plasmid Prep, Gradient PCR',
-
description: '<b>Members:</b> Rob, Andrew, Desmond<br> <b>What we did: </b>[Cl-] assay of the 87 clones<br><br>Chose 10 of the clones based on the results (5 representing each pathway) and set-up broths for a plasmid prep and a second [Cl-] assay (taking cells from plates instead of broth). '
+
start: new Date(2013, 8, 11),
-
},
+
description: 'Vivian, James, Desmond, Andrew<br>A gradient PCR was done on dhlB and dhlA from our positive GA samples.<br><br>Gels were run for each of our PCR products from the previous day.<br><br>The plasmid prep from earlier in the week was completed. Andrew later digested the Gibson assembly product using sspI. Desmond set up a digest for Rfp using ECRo1 and ran a gel of the digests.<br><br>Another PCR was done using the Gibson assembly digested fragments.'},
-
{
+
{ title: 'Ligation and Transformation',
-
title: 'Chloride Assay, Plasmid Prep',
+
start: new Date(2013, 8, 12),
-
start: new Date(2013, 7, 21),
+
description: 'Rob, Andrew, Vivian<br>Today a digestion of pSB-rfp was made using the enzymes, xbaI and PstI for ligation. Our PCR fragments (dhlA and dhlB) were also digested using the same restriction enzymes.<br><br>Following purification of our PCR DNA we ligated our inserts (dhlA, dhlB or dhlA-dhlB) into our plasmid vector (pSB). We split the reaction volume to two and use one later by storing in the cool room.<br><br>The ligated products were transformed into E.coli Top10 and EpI300 and plated on to LB-Cm.'},
-
description: '<b>Members:</b> Rob, Shuravi, Hugh<br> <b>What we did: </b>[Cl-] assayed the 10 clones. Plasmid prepped the 10 clones.'
+
{ title: 'PCR Screen',
-
},
+
start: new Date(2013, 8, 13),
-
{
+
description: 'Rob<br>We PCR screened for the correct dhlA, dhlB, dhlA-dhlB inserts by creating patch plates of white colonies on LB-Cm. Each clone was then mixed with EB and boiled to release DNA from cells. The cell suspension of each clone were used to PCR the DNA. Unfortunately some resulted in no PCR product.'},
-
title: 'Gel of Plasmid Prep',
+
{ title: 'Plasmid Prep, More Screening',
-
start: new Date(2013, 7, 22),
+
start: new Date(2013, 8, 14),
-
description: '<b>Members:</b> Rob, Nick<br> <b>What we did: </b>Ran a gel of yesterday’s plasmid prep and found it was too diluted and full of RNA.'
+
description: 'Rob, Andrew<br>Based on yesterday screens we selected clones for plasmid prepping. Plasmids were digested using EcoRV to check length and concentration of DNA.<br><br>To find successfully ligated dhlB we did more PCR screening. This time however we used EPI300 cells instead of TOP10. Screening was also done for dhlB-dhlA.'},
-
},
+
// -----------------Week 13 ----------------
-
{
+
{ title: 'Gel and Plasmid Prep (Again)',
-
title: 'Plasmid Prep Take 2',
+
start: new Date(2013, 8, 15),
-
start: new Date(2013, 7, 23),
+
description: 'Rob, Andrew, James<br>Following on from yesterdays digested plasmid prep a gel was run to at different concentrations.<br><br>We found, from the gel of our digest, that the plasmids were not concentrated enough.<br><br>Another plasmid prep, using some different clones was done. This time however, we incubated cells overnight to increase plasmid yield.<br><br>We digested and ran a gel of our plasmid for confirmation.<br><br><div style=\'color:red;font-weight:bold;\'>The gel turned out perfect!</div>'},
-
description: '<b>Members:</b> Viv<br> <b>What we did: </b>Treated plasmids with RNAse, repeated final steps of plasmid prep. '
+
{ title: 'Sending off Parts',
-
},
+
start: new Date(2013, 8, 16),
-
// -----------------Week 10 ----------------
+
description: 'Viv, James, Andrew, Rob<br>We sent off our parts for dhlA (BBa_K1115004), dhlB (BBa_K1115005) and dhlB-dhlA (BBa_K1115006), based on the results from PCR screening of cells and digests of plasmid preps.<br><br>However, we did a PCR screen using the plasmids as templates and discovered one of our parts is a reverse insert! This is dhlB (BBa_K1115005).'},
-
{
+
{ title: 'Sending off Parts, Characterisation',
-
title: 'Chloride Assay Prep',
+
start: new Date(2013, 8, 17),
-
start: new Date(2013, 7, 24),
+
description: 'Andrew, Rob<br>Re-submitted parts we’re pretty sure are correct. Started setting up cells and reagents for construction of a constitutive and inducible promoter system to characterise our parts in pSB1C#3 before the wiki-freeze.<br><br>PCR of parts directly from Distribution Kit for subsequent use in directional cloning.'},
-
end: new Date(2013, 7, 25),
+
{ title: 'Transformation and Promoter Hunting',
-
description: '<b>Members:</b> Andrew, Nick <br> <b>What we did: </b>- Plated out cells carrying pUC19-dhlB for positive control in [Cl-] assay. <br><br>- Inoculated 4ml broths for [Cl-] assay'
+
start: new Date(2013, 8, 18),
-
},
+
description: 'Rob, Shuravi, Viv, Andrew<br>Construction of Pcat-dhlB-dhlA in pSB1C3. Rob wrote out all the protocol and ran a digest, Viv ligated and transformed the construct, Shuravi spread-plated colonies.<br><br>Andrew went through a lot of troubleshooting trying to PCR parts or plasmid prep parts from the Distribution Kit for a lacI inducible promoter.'},
-
{
+
{ title: 'Screening Plates',
-
title: 'Chloride Assay',
+
start: new Date(2013, 8, 19),
-
start: new Date(2013, 7, 26),
+
description: 'Rob, Andrew<br>Figured out we could make screening plates to help us find transformants that are expressing our construct. We added chloroacetate and phenol red to LB-agar before plating and looked for colour change as the bacteria degraded chloroacetate and released Cl- ions.'},
-
description: '<b>Members:</b> Desmond<br> <b>What we did: </b>- Transferred overnight cultures (4mL) to fresh 50 mL LB and grown to an OD of ~1.0. Cells were harvested, cleaned and resuspended in 2mM chloroacetate for overnight incubation for chloride assay the next day.'
+
{ title: 'Promoter and Plate Construction',
-
},
+
start: new Date(2013, 8, 20),
-
{
+
description: 'Rob, Andrew<br>Construction of inducible promoter system in pSB1C3. Ran out of luck with lacI and turned to arabinose and tetracycline systems. PCR of parts from the Distribution Kit and verification of length and purity on gels.<br><br>Started playing around with the ingredients of chloroacetate-phenol red screening plates. We did a quick titration to find an optimal pH close to the colour-change from phenol red.'},
-
title: 'Chloride Assay Stuff',
+
{ title: 'Promoter Work, Selection Plates',
-
start: new Date(2013, 7, 27),
+
start: new Date(2013, 8, 21),
-
description: '<b>Members:</b> Rob<br> <b>What we did: </b>Remaining E.coli was spread plated onto Mackonkey agar for future negative Cl- assays.<br><br>Solutions for plasmid preps and chloride assays were made. We suspect the ambiguous plasmid prep and chloride assays results are due to poor stocks.'
+
end: new Date(2013, 8, 22),
-
},
+
description: 'Rob, Andrew, James, Viv<br>Sequential digestion and ligation of PCR products for an inducible promoter (Ptet and TetR, Pbad and AraC, parts from Distribution Kit).<br><br>Found that LB-agar-chloramphenicol plates with 10mM chloroacetate, 18mg/L phenol red, pH 6.8, worked best and allowed us to pick a few clones constitutively expressing dhlB for further characterisation by chloride assay.'},
-
{
+
{ title: 'Chloride Assay, Inducibility Screen',
-
title: 'Chloride Assay',
+
start: new Date(2013, 8, 23),
-
start: new Date(2013, 7, 28),
+
description: 'Rob, Andrew, Viv<br>Set-up chloride assay for a few promising clones constitutively expressing dhlB.<br><br>Set-up plates using the same screening system to find clones with inducible expression of dhlB.'},
-
description: '<b>Members:</b> Rob<br> <b>What we did: </b>Inoculated LB-Cm with our clones [2,10,38, 42,54,64, rfp(63)], LB-Am (positive control) and LB (negative control) for plasmid prep and chloride assay. No growth was observed in positive and negative control so no culture could be transferred for chloride assay.'
+
{ title: 'Chloride Assay',
-
},
+
start: new Date(2013, 8, 24),
-
{
+
description: 'Rob, Andrew<br>Chloride assay showed degradation of chloroacetate and DCA using the parts we submitted to the iGEM HQ.'},
-
title: 'Chloride Assay Stuff',
+
{ title: 'Triplicate Chloride Assay',
-
start: new Date(2013, 7, 29),
+
start: new Date(2013, 8, 25),
-
description: '<b>Members:</b> Rob, Shuravi, Desmond<br> <b>What we did: </b>Clones grown in LB-antibiotic broth overnight were washed and added to 2mM DCA reagents and another set in 2mM chloroacetate reagent.  Standards using NaCl solution was made simultaneously to ensure accuracy of the assay.<br><br>Plasmid preps were done using clones 2, 10, 38, 54, 42, 64 and rfp 63.<br><br>The samples were patch plated onto new LB-Cm plates.'
+
description: 'Rob, Andrew, James<br>Set-up another chloride assay in triplicate for neat characterisation of our parts, in parallel with promising clones with inducible-promoter systems.<br><br>James ran an SDS-page gel for further evidence that our parts are being expressed.'},
-
},
+
{ title: 'Chloride Assay, Promoter Characterisation',
-
// -----------------Week 11 ----------------
+
start: new Date(2013, 8, 26),
-
{
+
description: 'Rob, Andrew<br>Final chloride assay showed convincing degradation of chloroacetate and DCA using the parts we submitted to the iGEM HQ, also showed that our inducible-promoter systems failed to assemble correctly, instead containing just the constitutive promoter (Ptet). Andrew found further evidence for this by PCR screening.<br><br>Cleaned and packed up a lot of stuff in the lab.'},
-
title: 'Diagnostic Gel',
+
{ title: 'Wikifreeze',
-
start: new Date(2013, 7, 31),
+
start: new Date(2013, 8, 27),
-
description: '<b>Members:</b> Rob <br> <b>What we did: </b>A diagnostic digest was set up for clones 42, 54 and 64 using EcoRV and 2, 38, rfp using EcrIVHF. Banding patterns on our gel was difficult to see but was better visualised under UV.'
+
description: 'Everyone<br>Ohh no!! Wikifreeze!'},
-
},
+
{ title: 'Hong Kong Jamboree Preparation',
-
{
+
start: new Date(2013, 8, 30),
-
title: 'PCR Work',
+
        end: new Date(2013, 9, 2),
-
start: new Date(2013, 8, 2),
+
description: 'Everyone<br>Preparing our poster and presentation for HK.'},
-
description: '<b>Members:</b> Rob, James <br> <b>What we did: </b>Our new primers arrived. Today we PCR screened for dhlB and found the reverse primer corresponded to the synthetic dhlB sequence. Our PCR products were then loaded onto gel. The results were a little disappointing as there was no banding on our first gel and the ladder was difficult to see. Primer dimers were observed on our gel.<br><br>We also inoculated another 20 clones for screening from our initial Gibson Assembly transformation of p-p [contains p450] and p-a [contains adh] (These are our two different pathways).<br><br>We prepared some competent EPI400 cells. These are to be used later for the transformation of our GA products.'
+
{ title: 'Hong Kong Jamboree',
-
},
+
start: new Date(2013, 9, 4),
-
{
+
description: 'Everyone<br>Practice presentation until the early hours.'},
-
title: 'Cyril\'s Birthday',
+
{ title: 'Hong Kong Jamboree',
-
start: new Date(2013, 8, 2),
+
start: new Date(2013, 9, 5),
-
description: '<b>Members:</b> Cyril <br> <b>Happy Birthday :) </b>'
+
description: 'Everyone<br>Presentations all day!'},
-
},
+
{ title: 'Hong Kong Jamboree',
-
{
+
start: new Date(2013, 9, 6),
-
title: 'Cell Transformation, Gibson Assembly',
+
description: 'Everyone<br>Won the Best Human Practices and Best Experimental Measurement Approach!'},
-
start: new Date(2013, 8, 3),
+
{ title: 'Planning post-HK labwork',
-
description: '<b>Members:</b> Andrew, Rob <br> <b>What we did: </b>We transformed our Epi400 cells with our Gibson assembly products. Results did not look very promising. The Epi400 cells looked as they did when we transformed Epi300. The control worked and few cells grew with the positive Gibson assembly. There was more growth of cells transformed with p-p and p-a.<br><br>Another Gibson Assembly was set up for transformation. We found iGEMblock1 did not contain enough DNA leaving less than needed for the p-a sample.<br><br>We PCR screened for dhlB in colonies 100-139 however did not have a positive control (did not work yesterday). A gel was run for the dhlB PCR products.'
+
start: new Date(2013, 9, 9),
-
},
+
description: 'Rob, Andrew<br>Designing gBlocks and primers in Ho Chi Minh airport for labwork before MIT.'},
-
{
+
{ title: 'Ordering new gBlocks',
-
title: 'Cell Transformation',
+
start: new Date(2013, 9, 10),
-
start: new Date(2013, 8, 4),
+
description: 'Rob, Andrew<br>Convincing our supervisor to purchase the new gBlocks and primers we need.'},
-
description: '<b>Members:</b> Rob <br> <b>What we did: </b>Another transformation was performed using the second set of Gibson assembly products into E.coli TOP 10 and E.coli Epi400.  The transformed cells were plated onto the appropriate antibiotic media. '
+
{ title: 'Finding dhlB',
-
},
+
start: new Date(2013, 9, 11),
-
{
+
description: 'Hugh, Shuravi<br>Transformation of more clones with pSB1C3-dhlB ligation mixture. PCR Screen for correct orientation of dhlB from non-directional ligation. '},
-
title: 'PCR and Diagnostic Gel',
+
{ title: 'Isolating dhlB',
-
start: new Date(2013, 8, 5),
+
start: new Date(2013, 9, 12),
-
description: '<b>Members:</b> Andrew <br> <b>What we did: </b>We did a PCR of dhlB from the GA reaction products using three samples (p-p, p-a and a negative control containing no DNA)<br><br>All GA enzymes were heat-killed by placing using thermocycler at 95degres.<br><br>We ran a gel of dhlB PCR of Gibson assembly products. The resulting bands were clear and as expected.'
+
description: 'Andrew, Rob<br>Plasmid prep of promising clones containing pSB1C3-dhlB.'},
-
},
+
{ title: 'Confirming dhlB',
-
{
+
start: new Date(2013, 9, 13),
-
title: 'Diagnostic Gel',
+
description: 'Andrew<br>Digest confirmation of length and concentration of pSB1C3-dhlB.'},
-
start: new Date(2013, 8, 6),
+
{ title: 'Cloning dhlB',
-
description: '<b>Members:</b> Rob <br> <b>What we did: </b>A diagnostic digest was performed on our old plasmid preps. p-p was digested with BamH1, MluI, SmaI, SphI and Sal1. P-a digested with MluI, SmaI, SphI and rfp had no restriction enzyme added'
+
start: new Date(2013, 9, 14),
-
},
+
description: 'Rob<br>Cloning of the promoter Ptet (PCR product) into pSB1C3-dhlB.'},
-
// -----------------Week 12 ----------------
+
{ title: 'Confirming expression of dhlB',
-
{
+
start: new Date(2013, 9, 15),
-
title: 'Digests',
+
description: 'Rob, Desmond<br>Plating pSB1C3-Ptet-dhlB clones on pH-chloroacetate plates to find clones degrading chloroacetate. Set-up an overnight incubation of resting cells to confirm chloroacetate degradation.'},
-
start: new Date(2013, 8, 9),
+
{ title: 'Further confirmation',
-
description: '<b>Members:</b> Andrew, Desmond, Rob <br> <b>What we did: </b>Two digests were set up in parallel (p-p and p-a) using SspI and later purified using Quiaquick columns.'
+
start: new Date(2013, 9, 16),
-
},
+
description: 'James<br>Chloride assay to confirm chloroacetate degradation. Woo! We’ve got dhlB isolated and it works!'},
-
{
+
{ title: 'gBlocks arrived!',
-
title: 'Plasmid Prep, PCR Screen',
+
start: new Date(2013, 9, 17),
-
start: new Date(2013, 8, 10),
+
description: 'Rob, Andrew<br>gBlocks for p450, aldA and tetR arrived. Gibson Assembly and transformation.'},
-
description: '<b>Members:</b> Andrew <br> <b>What we did: </b>A plasmid prep was performed on pSB-RFP, taken from transformed E.coli TOP10 cells. Stopped at precipitation stage.<br><br>We received our new set of primers! We used these to PCR screen all our selected Gibson assembly plasmids and GA restriction products and our positive GA control (puc19-dhla-dhlb)<br><br>To confirm that our PCR screening had worked we ran a gel of all our PCR products'
+
{ title: 'Gibson transformation #1',
-
},
+
start: new Date(2013, 9, 18),
-
{
+
description: 'Andrew<br>Checked plates after Gibson Assembly - no colonies on tests and colonies on negative controls. Suspect bad plates. Remade plates and re-transformed Gibson reaction product.'},
-
title: 'Plasmid Prep, Gradient PCR',
+
{ title: 'PCR screening',
-
start: new Date(2013, 8, 11),
+
start: new Date(2013, 9, 19),
-
description: '<b>Members:</b> Vivian, James, Desmond, Andrew <br> <b>What we did: </b>A gradient PCR was done on dhlB and dhlA from our positive GA samples.<br><br>Gels were run for each of our PCR products from the previous day.<br><br>The plasmid prep from earlier in the week was completed. Andrew later digested the Gibson assembly product using sspI. Desmond set up a digest for Rfp using ECRo1 and ran a gel of the digests.<br><br>Another PCR was done using the Gibson assembly digested fragments.'
+
description: 'Rob<br>Checked plates again - better! Set-up a huge PCR screen for all Gibson constructs - aldA, p450 and tetR. Retransformed p450 Gibson reaction product to generate more clones for screening.'},
-
},
+
{ title: 'Plasmid prep',
-
{
+
start: new Date(2013, 9, 20),
-
title: 'Ligation and Transformation',
+
description: 'Rob, Andrew, Shuravi<br>More screening. Plasmid prep of promising clones.'},
-
start: new Date(2013, 8, 12),
+
{ title: 'Cloning',
-
description: '<b>Members:</b> Rob, Andrew, Vivian <br> <b>What we did: </b>Today a digestion of pSB-rfp was made using the enzymes, xbaI and PstI for ligation. Our PCR fragments (dhlA and dhlB) were also digested using the same restriction enzymes.<br><br>Following purification of our PCR DNA we ligated our inserts (dhlA, dhlB or dhla-dhlb) into our plasmid vector (pSB). We split the reaction volume to two and use one later by storing in the cool room.<br><br>The ligated products were transformed into E.coli Top10 and EpI300 and plated on to LB-Cm.'
+
start: new Date(2013, 9, 21),
-
},
+
description: 'Rob, Andrew, Hugh<br>Digest confirmation of plasmid with a RE specific to each gBlock. Confirmed length and concentration of all new parts. Digestion, gel purification, ligation and transformation of new parts so that they can be expressed.'},
-
{
+
{ title: 'Waiting for growth',
-
title: 'PCR Screen',
+
start: new Date(2013, 9, 22),
-
start: new Date(2013, 8, 13),
+
description: 'Andrew<br>Transformation plates hadn’t grown sufficiently for screening.'},
-
description: '<b>Members:</b> Rob <br> <b>What we did: </b>We PCR screened for the correct dhlA, dhlB, dhlA-dhlB inserts by creating patch plates of white colonies on LB-Cm. Each clone was then mixed with EB and boiled to release DNA from cells. The cell suspension of each clone were used to PCR the DNA. Unfortunately some resulted in no PCR product.'
+
{ title: 'Screening clones',
-
},
+
start: new Date(2013, 9, 23),
-
{
+
description: 'Rob, Hugh, Andrew<br>Patching and lysing cells from transformation plates for PCR screen and pH-chloroacetate screens. No efficient cloning for whole pathway, only for individual parts with tetR-inducible promoter system. Set-up chloride assay for degradation of DCA by clones containing tetR-p450 and tetR-aldA-dhlB-dhlA.'},
-
title: 'Plasmid Prep, More Screening',
+
{ title: 'Chloride assay',
-
start: new Date(2013, 8, 14),
+
start: new Date(2013, 9, 24),
-
description: '<b>Members:</b> Rob, Andrew <br> <b>What we did: </b>Based on yesterday screens we selected clones for plasmid prepping. Plasmids were digested using EcrOV to check length and concentration of DNA.<br><br>To find successfully ligated dhlB we did more PCR screening. This time however we used EPI300 cells instead of TOP10. Screening was also done for dlb-dhla.'
+
description: 'Rob, Andrew<br>Performed chloride assay. Appears there is reasonable degradation of DCA by p450.'},
-
},
+
{ title: 'Acetaldehyde growth inhibition',
-
// -----------------Week 13 ----------------
+
start: new Date(2013, 9, 25),
-
{
+
description: 'Rob, Andrew<br>Set-up an experiment to confirm aldA expression through growth inhibition of control E. coli in LB-acetaldehyde.'},
-
title: 'Gel and Plasmid Prep (Again)',
+
{ title: 'Characterising new parts',
-
start: new Date(2013, 8, 15),
+
start: new Date(2013, 9, 26),
-
description: '<b>Members:</b> Rob, Andrew, James <br> <b>What we did: </b>Following on from yesterdays digested plasmid prep a gel was run to at different concentrations.<br><br>We found, from the gel of our digest, that the plasmids were not concentrated enough.<br><br>Another plasmid prep, using some different clones was done. This time however, we incubated cells overnight to increase plasmid yield.<br><br>We digested and ran a gel of our plasmid for confirmation. <br><br><div style=\'color:red;font-weight:bold;\'>The gel turned out perfect!</div>'
+
description: 'Rob, Andrew<br>Another LB-acetaldehyde growth experiment in triplicate with a promising tetR-aldA clone. Incubated tetR-p450 clones with DCA in triplicate to confirm result from the 24th October, after 6 hours incubation, GC was not promising. Set-up an ethene-epoxide assay to confirm p450 expression.'},
-
},
+
{ title: 'Working on wiki',
-
{
+
start: new Date(2013, 9, 27),
-
title: 'Sending off Parts',
+
description: 'Viv, Rob, James, Hugh<br>Sat together and updated the wiki for changes to project made since Hong Kong'}
-
start: new Date(2013, 8, 16),
+
]    
-
description: '<b>Members:</b> Viv, James, Andrew, Rob <br> <b>What we did: </b>We sent off our parts for dhlA (BBa_K1115004), dhlB (BBa_K1115005) and dhlB-dhlA (BBa_K1115006), based on the results from PCR screening of cells and digests of plasmid preps.<br><br>However, we did a PCR screen using the plasmids as templates and discovered one of our parts is a reverse insert! This is dhlB (BBa_K1115005).'
+
-
},
+
-
{
+
-
title: 'Sending off Parts, Characterisation',
+
-
start: new Date(2013, 8, 17),
+
-
description: '<b>Members:</b> Andrew, Rob <br> <b>What we did: </b>Re-submitted parts we’re pretty sure are correct. Started setting up cells and reagents for construction of a constitutive and inducible promoter system to characterise our parts in pSB1C#3 before the wiki-freeze.<br><br>PCR of parts directly from Distribution Kit for subsequent use in directional cloning.'
+
-
},
+
-
{
+
-
title: 'Transformation and Promoter Hunting',
+
-
start: new Date(2013, 8, 18),
+
-
description: '<b>Members:</b> Rob, Shuravi, Viv, Andrew <br> <b>What we did: </b>Construction of Pcat-dhlB-dhlA in pSB1C3. Rob wrote out all the protocol and ran a digest, Viv ligated and transformed the construct, Shuravi spread-plated colonies.<br><br>Andrew went through a lot of troubleshooting trying to PCR parts or plasmid prep parts from the Distribution Kit for a lacI inducible promoter.'
+
-
},
+
-
{
+
-
title: 'Screening Plates',
+
-
start: new Date(2013, 8, 19),
+
-
description: '<b>Members:</b> Rob, Andrew <br> <b>What we did: </b>Figured out we could make screening plates to help us find transformants that are expressing our construct. We added chloroacetate and phenol red to LB-agar before plating and looked for colour change as the bacteria degraded chloroacetate and released Cl- ions.'
+
-
},
+
-
{
+
-
title: 'Promoter and Plate Construction',
+
-
start: new Date(2013, 8, 20),
+
-
description: '<b>Members:</b> Rob, Andrew <br> <b>What we did: </b>Construction of inducible promoter system in pSB1C3. Ran out of luck with lacI and turned to arabinose and tetracycline systems. PCR of parts from the Distribution Kit and verification of length and purity on gels.<br><br>Started playing around with the ingredients of chloroacetate-phenol red screening plates. We did a quick titration to find an optimal pH close to the colour-change from phenol red. '
+
-
},
+
-
{
+
-
title: 'Promoter Work, Selection Plates',
+
-
start: new Date(2013, 8, 21),
+
-
end: new Date(2013, 8, 22),
+
-
description: '<b>Members:</b> Rob, Andrew, James, Viv <br> <b>What we did: </b>Sequential digestion and ligation of PCR products for an inducible promoter (Ptet and TetR, Pbad and AraC, parts from Distribution Kit).<br><br>Found that LB-agar-chloramphenicol plates with 10mM chloroacetate, 18mg/L phenol red, pH 6.8, worked best and allowed us to pick a few clones constitutively expressing dhlB for further characterisation by chloride assay.'
+
-
},
+
-
{
+
-
title: 'Chloride Assay, Inducibility Screen',
+
-
start: new Date(2013, 8, 23),
+
-
description: '<b>Members:</b> Rob, Andrew, Viv <br> <b>What we did: </b>Set-up chloride assay for a few promising clones constitutively expressing dhlB.<br><br>Set-up plates using the same screening system to find clones with inducible expression of dhlB.'
+
-
},
+
-
{
+
-
title: 'Chloride Assay',
+
-
start: new Date(2013, 8, 24),
+
-
description: '<b>Members:</b> Rob, Andrew <br> <b>What we did: </b>Chloride assay showed degradation of chloroacetate and DCA using the parts we submitted to the iGEM HQ.'
+
-
},
+
-
{
+
-
title: 'Triplicate Chloride Assay',
+
-
start: new Date(2013, 8, 25),
+
-
description: '<b>Members:</b> Rob, Andrew, James <br> <b>What we did: </b>Set-up another chloride assay in triplicate for neat characterisation of our parts, in parallel with promising clones with inducible-promoter systems.<br><br>James ran an SDS-page gel for further evidence that our parts are being expressed.'
+
-
},
+
-
{
+
-
title: 'Chloride Assay, Promoter Characterisation',
+
-
start: new Date(2013, 8, 26),
+
-
description: '<b>Members:</b> Rob, Andrew <br> <b>What we did: </b>Final chloride assay showed convincing degradation of chloroacetate and DCA using the parts we submitted to the iGEM HQ, also showed that our inducible-promoter systems failed to assemble correctly, instead containing just the constitutive promoter (Ptet). Andrew found further evidence for this by PCR screening.<br><br>Cleaned and packed up a lot of stuff in the lab. '
+
-
},
+
-
+
-
{
+
-
title: 'Ignore this, I\'m testing :)',
+
-
start: new Date(y, m, 28),
+
-
end: new Date(y, m, 29),
+
-
url: 'http://google.com/'
+
-
}
+
-
]
+
-
                       
+
});
});
-
 
});
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Latest revision as of 00:49, 29 October 2013