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Team:Queens Canada/Notebook/Week16
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| - | <div id="protocolcontent"> | + | <div id="protocolcontent"><table class="tableizer-table"> |
| + | <tr class="tableizer-firstrow"><th>Date</th><th>Protocol</th><th>People</th><th>DNA (if relevant)</th><th>Quantities and Parameters (if relevant)</th><th>Notes on Protocol</th></tr> <tr><td>12-08-2012</td><td>PCR</td><td>Beini</td><td>GE pFliC1 + GFP + FliC2</td><td> </td><td> </td></tr> <tr><td>12-08-2012</td><td>Digestion with XS</td><td>Faisal </td><td>PCR products SmtA and fMt</td><td> </td><td>Fast Digest, enzymatic purification using Biobasic kit</td></tr> <tr><td>12-08-2012</td><td>PCR overlap extension of MBPs with FliC1</td><td>Faisal</td><td>SmtA, fMt, FliC1</td><td> </td><td> </td></tr> <tr><td>12-08-2012</td><td>Soft agar (0.25%) plates </td><td>Beini</td><td> </td><td>made 7 plates each of [C], [amp], [tet]</td><td> </td></tr> <tr><td>12-08-2012</td><td>Miniprep</td><td>Beini</td><td>K314100 high exp cassette, K314101 low exp cassette, K314103 lac expression cassette</td><td> </td><td> </td></tr> <tr><td>12-08-2012</td><td>Gel</td><td>Beini</td><td>K081005 SP GE, K314104 SP GE</td><td> </td><td> </td></tr> <tr><td>12-08-2012</td><td>Gel</td><td>Beini</td><td>nFF GFP GE, nFF GFP XP GE, pFF GFP XP GE, MPP K314100, MPP K314101, MPP K314103</td><td> </td><td> </td></tr> <tr><td>12-08-2012</td><td>Gel extraction</td><td>Kevin</td><td>nFF GFP, nFF GFP XP, pFF GFP XP, K081005 SP, K314104 SP</td><td> </td><td> </td></tr> <tr><td>12-08-2012</td><td>Gel</td><td>Kevin</td><td>MPP K081005, MPP K13104, pFF GFP, nFF GFP, pFF GFP XS</td><td> </td><td> </td></tr> <tr><td>12-08-2012</td><td>Digestions </td><td>Beini</td><td>"MPP K314100 with SP</td></tr> <tr><td>MPP K314103 with SP</td></tr> <tr><td>GE nFF GFP with XP"</td><td>digested MPPs for 12 mins, GEs for 30 mins</td><td> </td></tr> <tr><td>12-08-2012</td><td>Ligations</td><td>Kevin</td><td>pFF GFP in 1A2 from K088006</td><td>used 6 and 8 uL of vector for 1:1 and 3:1 ligations</td><td> </td></tr> <tr><td>12-08-2012</td><td>Gel </td><td>Kevin</td><td>1:1 lig, 3:1 lig, DIG XP nFF GFP, DIG SP K314100, DIG SP K314103</td><td> </td><td>gel extracted the digestions</td></tr> <tr><td>12-08-2012</td><td>Heat Shock Transformation using Motility Plates</td><td>Kevin</td><td> </td><td> </td><td> </td></tr> <tr><td>13-08-2012</td><td>Ligations</td><td>Victor</td><td>"nFF GFP XP GE + 1A3 XP GE</td></tr> <tr><td>nFF GFP XP GE + 1A3 XP GE</td></tr> <tr><td>nFF GFP XP GE + T7 GE SP</td></tr> <tr><td>nFF GFP XP GE + K314100 GE SP</td></tr> <tr><td>nFF GFP ctrl"</td><td> </td><td> </td></tr> <tr><td>13-08-2012</td><td>Gel</td><td>David, Kevin</td><td>fMT FliC, SmA FliC, DIG nFF GFP XP, LIG nFF GFP XP 1A3, LIG nFF GFP XP T7, LIG nFF GFP XP K314100</td><td> </td><td> </td></tr> <tr><td>13-08-2012</td><td>Digestions </td><td>Victor</td><td>nFF GFP GE (3) with XP</td><td> </td><td> </td></tr> <tr><td>13-08-2012</td><td>Gel extraction</td><td>David</td><td>fMt FliC, SmtA FliC from above gel</td><td> </td><td> </td></tr> <tr><td>13-08-2012</td><td>Gel</td><td>Kevin</td><td>nFF GFP XP, K314100 SP, SmtA FliC1, fMt FliC1</td><td> </td><td> </td></tr> <tr><td>13-08-2012</td><td>Ligations</td><td>Kevin</td><td>"Vectors: K314104, K081005, K314100, K314003, J04500</td></tr> <tr><td>Insert: nFF GFP XP"</td><td>1:1, 2:1 insert:vector ratios</td><td>plated 100 uL on [K], 100 uL on [AK], spun down the rest at 12000 rpm and resuspended 100 uL on [AK]</td></tr> <tr><td>13-08-2012</td><td>Digestions </td><td>Beini</td><td>"MPP J33204 xylE + RBS with XP</td></tr> <tr><td>nFF GFP GE with XP"</td><td>"digested MPP for 13 mins at 37C</td></tr> <tr><td>digested GEs for 30 mins at 37C"</td><td>iced while waiting for 80C bath to heat up</td></tr> <tr><td>14-08-2012</td><td>Liquid cultures </td><td>Kevin</td><td>pFF GFP 1A3 1:3 lig (the rest) </td><td> </td><td> </td></tr> <tr><td>14-08-2012</td><td>Digestions </td><td>David </td><td>GEs SmtA + FliC, fMt + FliC1 with SpeI</td><td> </td><td> </td></tr> <tr><td>14-08-2012</td><td>Digestions </td><td>Victor</td><td>nFF GFP GE with XP</td><td> </td><td> </td></tr> <tr><td>14-08-2012</td><td>Digestions of linearized plasmid backbone</td><td>Victor</td><td>pSB1C3, pSB1A3 with XP and DpnI</td><td> </td><td>digestion purification</td></tr> <tr><td>14-08-2012</td><td>Gel Extraction</td><td>Victor</td><td>DIG XP nFF GFP, npp pFF GFP 1A3, DIG EP pFF GFP 1A3, pSB1C3 XP </td><td> </td><td>did enzymatic purification of pSB1C3 digest instead of gel purification</td></tr> <tr><td>14-08-2012</td><td>Gel Extraction</td><td>Kevin</td><td>nFF GFP XP, nFF GFP XP, DIG xylE + RBS XP</td><td> </td><td> </td></tr> <tr><td>14-08-2012</td><td>Miniprep</td><td>Kevin</td><td>LIG pFF GFP + 1A3 1:3 (the rest)</td><td> </td><td> </td></tr> <tr><td>14-08-2012</td><td>Digestion</td><td>Kevin</td><td>LIG pFF GFP + 1A3 1:3 (the rest) with EP</td><td> </td><td> </td></tr> <tr><td>14-08-2012</td><td>PCR overlap extension</td><td>Faisal</td><td>fliC1 + MBP, fliC2</td><td>did 1:1, 2:1, 3:1 ratios of fliC1 + MBP : fliC2</td><td>digestion purification of SmtA + fliC1 and fMT + fliC1 digested with SpeI</td></tr> <tr><td>14-08-2012</td><td>Ligations</td><td>Victor, Mitangi</td><td>pSB1A3 + nFF GFP</td><td>did 1:1, 2:1 ratios of insert : vector</td><td> </td></tr> <tr><td>14-08-2012</td><td>Gel to check for concentrations</td><td>Victor</td><td>nFF GFP GE XP, nFF GFP GE XP, GE xylE + RBS XP plasmid, GE xylE + RBS</td><td> </td><td> </td></tr> <tr><td>14-08-2012</td><td>Liquid cultures of fluorescent colonies</td><td>Kevin, Faisal</td><td>nFF GFP + J04500 (6 trials + 3 ctrls)</td><td>"# of fluorescent colonies </td></tr> <tr><td>AK 1:1 100 uL - 10</td></tr> <tr><td>AK 1:1 the rest - 21</td></tr> <tr><td>K 1:1 100 uL - 50</td></tr> <tr><td>AK: 1:3 100 uL - 0</td></tr> <tr><td>AK 1:3 the rest - 2</td></tr> <tr><td>K 1:3 100 uL - 2"</td><td> </td></tr> <tr><td>14-08-2012</td><td>Heat shock transformation</td><td>Beini</td><td>nFF GFP + 1A3 </td><td>1:1, 2:1, ctrl</td><td> </td></tr> <tr><td>14-08-2012</td><td>Gel extraction</td><td>Faisal, David</td><td>fmt FliC1 + FliC2, SmtA FliC1 + FliC2</td><td> </td><td> </td></tr> <tr><td>15-08-2012</td><td>Minipreps</td><td>Kevin</td><td>nFF GFP + J04500 6 trials, pFF GFP 1A3 1:1 the rest</td><td> </td><td> </td></tr> <tr><td>15-08-2012</td><td>PCR of Full FliC MBP Gel Extractions</td><td>David, Faisal</td><td>fmt FliC1 + FliC2, SmtA FliC1 + FliC2</td><td> </td><td> </td></tr> <tr><td>15-08-2012</td><td>Digestion</td><td>Phillip</td><td>nFF GFP + J04500 6 trials, pFF GFP 1A3 1:1 the rest with ES</td><td> </td><td> </td></tr> <tr><td>15-08-2012</td><td>Gel</td><td>Victor</td><td>"DIG B0015 EX</td></tr> <tr><td>DIG B0017 EX</td></tr> <tr><td>DIG nFF GFP + J04500 ES</td></tr> <tr><td>pFF GFP + 1A3</td></tr> <tr><td>MPP nFF GFP + J04506</td></tr> <tr><td>MPP nFF GFP + J04560"</td><td> </td><td> </td></tr> <tr><td>15-08-2012</td><td>Ligations</td><td>Victor</td><td>GE nFF GFP XP, 1C3 XP GE</td><td>did 1:1, 2:1 insert:vector ratios </td><td> </td></tr> <tr><td>15-08-2012</td><td>Gel</td><td>Phillip</td><td>"MPP nFF + J04500</td></tr> <tr><td>MPP pFF GFP 1A3"</td><td> </td><td> </td></tr> <tr><td>15-08-2012</td><td>Liquid culture</td><td>Phillip</td><td>nFF GFP + 1A3 </td><td> </td><td> </td></tr> <tr><td>15-08-2012</td><td>Streak plating</td><td>Victor</td><td>nFF GFP + J04500 </td><td>1:2, 1:3, 1:1</td><td> </td></tr> <tr><td>15-08-2012</td><td>Gel Extraction of FF MBP products from PCR overlap extension</td><td>Faisal</td><td>SmtA FliC1 + FliC2</td><td> </td><td> </td></tr> <tr><td>15-08-2012</td><td>Digestioin</td><td>Victor</td><td>B0015, B0017 terminators with EX</td><td> </td><td> </td></tr> <tr><td>15-08-2012</td><td>PCR overlap extension</td><td>Kevin</td><td>mCer DP XS, nFF GFP + J04500</td><td>"need a super high insert:vector ratio, >>50:1</td></tr> <tr><td>extension time 5 min 30 s, 17 cycles"</td><td> </td></tr> <tr><td>15-08-2012</td><td>Liquid Culture</td><td>Kevin</td><td>nFFGFP 1A3 4 trials, J04500</td><td> </td><td> </td></tr> <tr><td>15-08-2012</td><td>Motility plate inoculation </td><td>Kevin</td><td>nFF GFP + J04500 6 trials</td><td>3 uL stab + inject per spot</td><td>1 stop only on pipette</td></tr> <tr><td>15-08-2012</td><td>Digestion of mCer OE </td><td>Kevin</td><td>mCer OE</td><td>17 uL DNA, 1 uL DpnI, 2 uL buffer Tango</td><td> </td></tr> <tr><td>16-08-2012</td><td>Digestion of PP mCer and PP mCit with XS</td><td>David</td><td>PP mCer, PP mCit</td><td> </td><td>ran out of SpeI, only got a bit of S for mCit1; mCer2 and mCit2 with X only</td></tr> <tr><td>16-08-2012</td><td>Ligations</td><td>Victor</td><td>GE nFF GFP XP + 1C3 XP GE from Antigen-43</td><td>1:1 insert:vector</td><td> </td></tr> <tr><td>16-08-2012</td><td>Digestion</td><td>Victor</td><td>Luciferase PCR products with XS </td><td> </td><td> </td></tr> <tr><td>16-08-2012</td><td>Miniprep</td><td>Kevin</td><td>nFF GFP + 1A3, J04500, nFF GFP + 1A3, nFF GFP + 1A3</td><td> </td><td> </td></tr> <tr><td>16-08-2012</td><td>Digestion with EP</td><td>Kevin</td><td>nFF GFP + 1A3, nFF GFP + 1A3, nFF GFP + 1A3</td><td>digested 10 uL of dna</td><td>NEB </td></tr> <tr><td>16-08-2012</td><td>Gel extraction</td><td>Victor, Beini</td><td>"DIG mCer XS, DIG mCer X, dig mCit XS, DIG mCit X, DIG luciferase XS</td></tr> <tr><td>gelled to check concs: GE nFF GFP XP, GE xylE + RBS XP plasmid, GE xylE + RBS XP"</td><td> </td><td>DIG mCit XS did not show up on gel</td></tr> <tr><td>16-08-2012</td><td>Gel</td><td>Kevin</td><td>MPP nff GFP 2:1 the rest, DIG EP nFF GFP 2:1 the rest, MPP J04500, MPP nFF GFP 1A3, DIG EP nFF GFP 1A3</td><td> </td><td> </td></tr> <tr><td>16-08-2012</td><td>Digestion w/ EcoRI-HF</td><td>Kevin</td><td>MPP nFF GFP 1A3 2:1 the rest</td><td> </td><td> </td></tr> <tr><td>16-08-2012</td><td>Gel</td><td>Kevin</td><td>GE mCer X, GE luciferase XS, DIG nFF GFP E</td><td> </td><td> </td></tr> <tr><td>16-08-2012</td><td>PCR overlap extension</td><td>Kevin</td><td>"inserts: mCer, luciferase</td></tr> <tr><td>vector: nFF GFP + J04500 K"</td><td>8 mins. 30 s extension time, 18 cycles</td><td>1 trial with Kapa, 1 trial with Phusion</td></tr> <tr><td>16-08-2012</td><td>Liquid cultures</td><td>Kevin</td><td>fluorescent colony AK nFF GFP J04500 1:3 the rest from 08/14 streak plate</td><td> </td><td> </td></tr> <tr><td>16-08-2012</td><td>Spectrometer </td><td>Kevin</td><td> </td><td>"OD600</td></tr> <tr><td>2XTY against no reference: 0.055</td></tr> <tr><td>J04500 culture: 1.878</td></tr> <tr><td>nFF GFP + J04500 1:2 K: 1.701 (using a different cuvette = 1.731)</td></tr> <tr><td>nFF GFP + J04500 1:2 AK: 1.760"</td><td> </td></tr> <tr><td>16-08-2012</td><td>Motility plate inoculations</td><td>Kevin</td><td>J04500, nFF GFP + J04500 1:2 K, nFF GFP + J04500 1:2 AK </td><td>only J04500 shows motility</td><td> </td></tr> <tr><td>16-08-2012</td><td>Gel</td><td>Phillip</td><td>PCR-OE products: luciferase Kapa, luciferase Phusion</td><td> </td><td> </td></tr> <tr><td>17-08-2012</td><td>250 mL inoculations of 2XTY</td><td>Victor</td><td> AK nFF GFP + J04500 1:2, AK J04500 </td><td> </td><td> </td></tr> <tr><td>17-08-2012</td><td>Digestions with DpnI using Tango buffer</td><td>Phillip</td><td>PCR-OE products: luciferase Kapa, luciferase Phusion</td><td> </td><td> </td></tr> <tr><td>17-08-2012</td><td>Using the ultracentrifuge to obtain a bacterial cell pellet</td><td>Victor, as told by Jun </td><td> </td><td> </td><td>"use JA-10 rotor and 250 mL bottles</td></tr> <tr><td>10 000 rpm, 6000 speed, 10 mins., 4C"</td></tr> <tr><td>17-08-2012</td><td>Tris-HCl buffer</td><td>Victor</td><td> </td><td>"12.1 g Tris, 800 mL H2O, 7.7 mL HCl until pH 7.8 is reached, fill the rest to 1 L of solution</td></tr> <tr><td>autoclave at Liquid 1 setting"</td><td> </td></tr> <tr><td>17-08-2012</td><td>Liquid culture of ligations</td><td>Beini</td><td>nFF GFP 1C3 100 pellet, nFF GFP 1C3 100 uL, nFF GFP 1A2 1:1 pellet, nFF GFP 1A2 1:1 100 uL</td><td> </td><td> </td></tr> <tr><td>18-08-2012</td><td>Isolation of flagella</td><td>Beini</td><td>AK nFF GFP + J04500 1:2, AK J04500 </td><td> </td><td>"resuspended cell pellet in 100 mL Tris-HCl</td></tr> <tr><td>blended 1 min 30 s in Waring blender at 4C</td></tr> <tr><td>centrifuged 10 mins. at 4C, 10 000 rpm, speed 6000 </td></tr> <tr><td>centrifuged supernatant for 1 h at 4C, 20 000 rpm, speed 6000"</td></tr> <tr><td>18-08-2012</td><td>Liquid cultures</td><td>Mitangi</td><td>AK DIG luciferase Kapa DpnI</td><td> </td><td> </td></tr> <tr><td>18-08-2012</td><td>Miniprep</td><td>Mitangi</td><td>nFF GFP 1A2, nFF GFP 1C3</td><td> </td><td> </td></tr> <tr><td>18-08-2012</td><td>Digestion with PstI</td><td>Mitangi</td><td>nFF GFP 1A2, nFF GFP 1C3, nFF GFP 1A3 (all MPPs)</td><td> </td><td> </td></tr> <tr><td>18-08-2012</td><td>Gel</td><td>Beini</td><td>MPP nFF GFP 1A3, DIG P nFF GFP 1A3, MPP nFF GFP 1A2, DIG nFF GFP 1A2 P, MPP nFF GFP 1A2, DIG P nFF GFP 1C3, DIG P nFF GFO 1C3</td><td> </td><td> </td></tr> <tr><td>18-08-2012</td><td>Miniprep</td><td>Beini</td><td>AK nFF GFP J04500 1:3 the rest</td><td> </td><td>made glycerol stock</td></tr> <tr><td>18-08-2012</td><td>Miniprep</td><td>Beini</td><td>AK DIG luciferase Kapa DpnI (PCR OE of luciferase + nFF GFP J04500)</td><td> </td><td></td></tr></table> | ||
| + | </div> | ||
<div id="notebookcontent"> | <div id="notebookcontent"> | ||
<p style="font-size: 2em; text-align:middle'"> Given that the vast majority of our work now is in the lab, we will only be updating the "Labwork" section of the Notebook. </p> | <p style="font-size: 2em; text-align:middle'"> Given that the vast majority of our work now is in the lab, we will only be updating the "Labwork" section of the Notebook. </p> | ||
Revision as of 03:55, 4 October 2012
Control
Notebook - Week 1
| Date | Protocol | People | DNA (if relevant) | Quantities and Parameters (if relevant) | Notes on Protocol |
|---|---|---|---|---|---|
| 12-08-2012 | PCR | Beini | GE pFliC1 + GFP + FliC2 | ||
| 12-08-2012 | Digestion with XS | Faisal | PCR products SmtA and fMt | Fast Digest, enzymatic purification using Biobasic kit | |
| 12-08-2012 | PCR overlap extension of MBPs with FliC1 | Faisal | SmtA, fMt, FliC1 | ||
| 12-08-2012 | Soft agar (0.25%) plates | Beini | made 7 plates each of [C], [amp], [tet] | ||
| 12-08-2012 | Miniprep | Beini | K314100 high exp cassette, K314101 low exp cassette, K314103 lac expression cassette | ||
| 12-08-2012 | Gel | Beini | K081005 SP GE, K314104 SP GE | ||
| 12-08-2012 | Gel | Beini | nFF GFP GE, nFF GFP XP GE, pFF GFP XP GE, MPP K314100, MPP K314101, MPP K314103 | ||
| 12-08-2012 | Gel extraction | Kevin | nFF GFP, nFF GFP XP, pFF GFP XP, K081005 SP, K314104 SP | ||
| 12-08-2012 | Gel | Kevin | MPP K081005, MPP K13104, pFF GFP, nFF GFP, pFF GFP XS | ||
| 12-08-2012 | Digestions | Beini | "MPP K314100 with SP | ||
| MPP K314103 with SP | |||||
| GE nFF GFP with XP" | digested MPPs for 12 mins, GEs for 30 mins | ||||
| 12-08-2012 | Ligations | Kevin | pFF GFP in 1A2 from K088006 | used 6 and 8 uL of vector for 1:1 and 3:1 ligations | |
| 12-08-2012 | Gel | Kevin | 1:1 lig, 3:1 lig, DIG XP nFF GFP, DIG SP K314100, DIG SP K314103 | gel extracted the digestions | |
| 12-08-2012 | Heat Shock Transformation using Motility Plates | Kevin | |||
| 13-08-2012 | Ligations | Victor | "nFF GFP XP GE + 1A3 XP GE | ||
| nFF GFP XP GE + 1A3 XP GE | |||||
| nFF GFP XP GE + T7 GE SP | |||||
| nFF GFP XP GE + K314100 GE SP | |||||
| nFF GFP ctrl" | |||||
| 13-08-2012 | Gel | David, Kevin | fMT FliC, SmA FliC, DIG nFF GFP XP, LIG nFF GFP XP 1A3, LIG nFF GFP XP T7, LIG nFF GFP XP K314100 | ||
| 13-08-2012 | Digestions | Victor | nFF GFP GE (3) with XP | ||
| 13-08-2012 | Gel extraction | David | fMt FliC, SmtA FliC from above gel | ||
| 13-08-2012 | Gel | Kevin | nFF GFP XP, K314100 SP, SmtA FliC1, fMt FliC1 | ||
| 13-08-2012 | Ligations | Kevin | "Vectors: K314104, K081005, K314100, K314003, J04500 | ||
| Insert: nFF GFP XP" | 1:1, 2:1 insert:vector ratios | plated 100 uL on [K], 100 uL on [AK], spun down the rest at 12000 rpm and resuspended 100 uL on [AK] | |||
| 13-08-2012 | Digestions | Beini | "MPP J33204 xylE + RBS with XP | ||
| nFF GFP GE with XP" | "digested MPP for 13 mins at 37C | ||||
| digested GEs for 30 mins at 37C" | iced while waiting for 80C bath to heat up | ||||
| 14-08-2012 | Liquid cultures | Kevin | pFF GFP 1A3 1:3 lig (the rest) | ||
| 14-08-2012 | Digestions | David | GEs SmtA + FliC, fMt + FliC1 with SpeI | ||
| 14-08-2012 | Digestions | Victor | nFF GFP GE with XP | ||
| 14-08-2012 | Digestions of linearized plasmid backbone | Victor | pSB1C3, pSB1A3 with XP and DpnI | digestion purification | |
| 14-08-2012 | Gel Extraction | Victor | DIG XP nFF GFP, npp pFF GFP 1A3, DIG EP pFF GFP 1A3, pSB1C3 XP | did enzymatic purification of pSB1C3 digest instead of gel purification | |
| 14-08-2012 | Gel Extraction | Kevin | nFF GFP XP, nFF GFP XP, DIG xylE + RBS XP | ||
| 14-08-2012 | Miniprep | Kevin | LIG pFF GFP + 1A3 1:3 (the rest) | ||
| 14-08-2012 | Digestion | Kevin | LIG pFF GFP + 1A3 1:3 (the rest) with EP | ||
| 14-08-2012 | PCR overlap extension | Faisal | fliC1 + MBP, fliC2 | did 1:1, 2:1, 3:1 ratios of fliC1 + MBP : fliC2 | digestion purification of SmtA + fliC1 and fMT + fliC1 digested with SpeI |
| 14-08-2012 | Ligations | Victor, Mitangi | pSB1A3 + nFF GFP | did 1:1, 2:1 ratios of insert : vector | |
| 14-08-2012 | Gel to check for concentrations | Victor | nFF GFP GE XP, nFF GFP GE XP, GE xylE + RBS XP plasmid, GE xylE + RBS | ||
| 14-08-2012 | Liquid cultures of fluorescent colonies | Kevin, Faisal | nFF GFP + J04500 (6 trials + 3 ctrls) | "# of fluorescent colonies | |
| AK 1:1 100 uL - 10 | |||||
| AK 1:1 the rest - 21 | |||||
| K 1:1 100 uL - 50 | |||||
| AK: 1:3 100 uL - 0 | |||||
| AK 1:3 the rest - 2 | |||||
| K 1:3 100 uL - 2" | |||||
| 14-08-2012 | Heat shock transformation | Beini | nFF GFP + 1A3 | 1:1, 2:1, ctrl | |
| 14-08-2012 | Gel extraction | Faisal, David | fmt FliC1 + FliC2, SmtA FliC1 + FliC2 | ||
| 15-08-2012 | Minipreps | Kevin | nFF GFP + J04500 6 trials, pFF GFP 1A3 1:1 the rest | ||
| 15-08-2012 | PCR of Full FliC MBP Gel Extractions | David, Faisal | fmt FliC1 + FliC2, SmtA FliC1 + FliC2 | ||
| 15-08-2012 | Digestion | Phillip | nFF GFP + J04500 6 trials, pFF GFP 1A3 1:1 the rest with ES | ||
| 15-08-2012 | Gel | Victor | "DIG B0015 EX | ||
| DIG B0017 EX | |||||
| DIG nFF GFP + J04500 ES | |||||
| pFF GFP + 1A3 | |||||
| MPP nFF GFP + J04506 | |||||
| MPP nFF GFP + J04560" | |||||
| 15-08-2012 | Ligations | Victor | GE nFF GFP XP, 1C3 XP GE | did 1:1, 2:1 insert:vector ratios | |
| 15-08-2012 | Gel | Phillip | "MPP nFF + J04500 | ||
| MPP pFF GFP 1A3" | |||||
| 15-08-2012 | Liquid culture | Phillip | nFF GFP + 1A3 | ||
| 15-08-2012 | Streak plating | Victor | nFF GFP + J04500 | 1:2, 1:3, 1:1 | |
| 15-08-2012 | Gel Extraction of FF MBP products from PCR overlap extension | Faisal | SmtA FliC1 + FliC2 | ||
| 15-08-2012 | Digestioin | Victor | B0015, B0017 terminators with EX | ||
| 15-08-2012 | PCR overlap extension | Kevin | mCer DP XS, nFF GFP + J04500 | "need a super high insert:vector ratio, >>50:1 | |
| extension time 5 min 30 s, 17 cycles" | |||||
| 15-08-2012 | Liquid Culture | Kevin | nFFGFP 1A3 4 trials, J04500 | ||
| 15-08-2012 | Motility plate inoculation | Kevin | nFF GFP + J04500 6 trials | 3 uL stab + inject per spot | 1 stop only on pipette |
| 15-08-2012 | Digestion of mCer OE | Kevin | mCer OE | 17 uL DNA, 1 uL DpnI, 2 uL buffer Tango | |
| 16-08-2012 | Digestion of PP mCer and PP mCit with XS | David | PP mCer, PP mCit | ran out of SpeI, only got a bit of S for mCit1; mCer2 and mCit2 with X only | |
| 16-08-2012 | Ligations | Victor | GE nFF GFP XP + 1C3 XP GE from Antigen-43 | 1:1 insert:vector | |
| 16-08-2012 | Digestion | Victor | Luciferase PCR products with XS | ||
| 16-08-2012 | Miniprep | Kevin | nFF GFP + 1A3, J04500, nFF GFP + 1A3, nFF GFP + 1A3 | ||
| 16-08-2012 | Digestion with EP | Kevin | nFF GFP + 1A3, nFF GFP + 1A3, nFF GFP + 1A3 | digested 10 uL of dna | NEB |
| 16-08-2012 | Gel extraction | Victor, Beini | "DIG mCer XS, DIG mCer X, dig mCit XS, DIG mCit X, DIG luciferase XS | ||
| gelled to check concs: GE nFF GFP XP, GE xylE + RBS XP plasmid, GE xylE + RBS XP" | DIG mCit XS did not show up on gel | ||||
| 16-08-2012 | Gel | Kevin | MPP nff GFP 2:1 the rest, DIG EP nFF GFP 2:1 the rest, MPP J04500, MPP nFF GFP 1A3, DIG EP nFF GFP 1A3 | ||
| 16-08-2012 | Digestion w/ EcoRI-HF | Kevin | MPP nFF GFP 1A3 2:1 the rest | ||
| 16-08-2012 | Gel | Kevin | GE mCer X, GE luciferase XS, DIG nFF GFP E | ||
| 16-08-2012 | PCR overlap extension | Kevin | "inserts: mCer, luciferase | ||
| vector: nFF GFP + J04500 K" | 8 mins. 30 s extension time, 18 cycles | 1 trial with Kapa, 1 trial with Phusion | |||
| 16-08-2012 | Liquid cultures | Kevin | fluorescent colony AK nFF GFP J04500 1:3 the rest from 08/14 streak plate | ||
| 16-08-2012 | Spectrometer | Kevin | "OD600 | ||
| 2XTY against no reference: 0.055 | |||||
| J04500 culture: 1.878 | |||||
| nFF GFP + J04500 1:2 K: 1.701 (using a different cuvette = 1.731) | |||||
| nFF GFP + J04500 1:2 AK: 1.760" | |||||
| 16-08-2012 | Motility plate inoculations | Kevin | J04500, nFF GFP + J04500 1:2 K, nFF GFP + J04500 1:2 AK | only J04500 shows motility | |
| 16-08-2012 | Gel | Phillip | PCR-OE products: luciferase Kapa, luciferase Phusion | ||
| 17-08-2012 | 250 mL inoculations of 2XTY | Victor | AK nFF GFP + J04500 1:2, AK J04500 | ||
| 17-08-2012 | Digestions with DpnI using Tango buffer | Phillip | PCR-OE products: luciferase Kapa, luciferase Phusion | ||
| 17-08-2012 | Using the ultracentrifuge to obtain a bacterial cell pellet | Victor, as told by Jun | "use JA-10 rotor and 250 mL bottles | ||
| 10 000 rpm, 6000 speed, 10 mins., 4C" | |||||
| 17-08-2012 | Tris-HCl buffer | Victor | "12.1 g Tris, 800 mL H2O, 7.7 mL HCl until pH 7.8 is reached, fill the rest to 1 L of solution | ||
| autoclave at Liquid 1 setting" | |||||
| 17-08-2012 | Liquid culture of ligations | Beini | nFF GFP 1C3 100 pellet, nFF GFP 1C3 100 uL, nFF GFP 1A2 1:1 pellet, nFF GFP 1A2 1:1 100 uL | ||
| 18-08-2012 | Isolation of flagella | Beini | AK nFF GFP + J04500 1:2, AK J04500 | "resuspended cell pellet in 100 mL Tris-HCl | |
| blended 1 min 30 s in Waring blender at 4C | |||||
| centrifuged 10 mins. at 4C, 10 000 rpm, speed 6000 | |||||
| centrifuged supernatant for 1 h at 4C, 20 000 rpm, speed 6000" | |||||
| 18-08-2012 | Liquid cultures | Mitangi | AK DIG luciferase Kapa DpnI | ||
| 18-08-2012 | Miniprep | Mitangi | nFF GFP 1A2, nFF GFP 1C3 | ||
| 18-08-2012 | Digestion with PstI | Mitangi | nFF GFP 1A2, nFF GFP 1C3, nFF GFP 1A3 (all MPPs) | ||
| 18-08-2012 | Gel | Beini | MPP nFF GFP 1A3, DIG P nFF GFP 1A3, MPP nFF GFP 1A2, DIG nFF GFP 1A2 P, MPP nFF GFP 1A2, DIG P nFF GFP 1C3, DIG P nFF GFO 1C3 | ||
| 18-08-2012 | Miniprep | Beini | AK nFF GFP J04500 1:3 the rest | made glycerol stock | |
| 18-08-2012 | Miniprep | Beini | AK DIG luciferase Kapa DpnI (PCR OE of luciferase + nFF GFP J04500) |
Given that the vast majority of our work now is in the lab, we will only be updating the "Labwork" section of the Notebook.
