Team:Lethbridge/Notebook
From 2009.igem.org
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(→May 29) |
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</body> | </body> | ||
</html> | </html> | ||
+ | |||
+ | == June == | ||
+ | ===June 1=== | ||
+ | |||
+ | '''Roxanne''' | ||
+ | |||
+ | *Ran a 1% agarose in TAE gel of the PCR products from May 28th. | ||
+ | *5µL of ladder, 2µL of DNA | ||
+ | |||
+ | Lane 1: ladder | ||
+ | |||
+ | Lane 2: ohbA (conc.1x) | ||
+ | |||
+ | Lane 3: ohbA (conc.1/10) | ||
+ | |||
+ | Lane 4: ohbB(1x) | ||
+ | |||
+ | Lane 5: ohbB(1/10) | ||
+ | |||
+ | Lane 6: ohbC(1x) | ||
+ | |||
+ | Lane 7: ohbC(1/10) | ||
+ | |||
+ | Lane 8: ohbR (1x) | ||
+ | |||
+ | Lane 9: ohbR(1/10) | ||
+ | |||
+ | Lane 10: ohbR(1x) | ||
+ | |||
+ | *Gel did not show any amplification | ||
+ | |||
+ | Mackenzie & Roxanne | ||
+ | |||
+ | *Transformation of pSB1A3 into DH5α | ||
+ | |||
+ | *Made 2 aliquots of pSB1A3 and 1 of pUC19 | ||
+ | |||
+ | *plated pSB1A3-1: straight and dilute, pSB1A3-2: straight and dilute, pUC19: straight only incubated overnight at 37°C | ||
+ | |||
+ | ===June 3=== | ||
+ | '''Roxanne''' | ||
+ | |||
+ | *positive control worked | ||
+ | *Think the transformation worked but slight problem. The plasmid contains a suicide gene. Therefore, any cells that took up the plasmid would die. | ||
+ | *planning new genes to transform | ||
+ | *GENE LOCATION pSB1A3 + IPTG Inducible RFP 1-1k Bba_I13522, pTET GFP 2-8A Bba_I13521, pTet mRFP 2-6O Bba_I13600, pTET CFP 1-24E BBA-B0015, double terminator 1-23L | ||
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+ | </head> | ||
+ | <body> | ||
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+ | |||
+ | <li><a href="https://2009.igem.org/Team:Lethbridge">Home</a></li> | ||
+ | <li><a href="https://2009.igem.org/Team:Lethbridge/Notebook">Top of Page</a></li> | ||
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+ | |||
+ | ===June 4=== | ||
+ | |||
+ | *Picked some glycerol stock GFP for the AIF visit | ||
+ | |||
+ | *made ampicillin plates 371.39g/mol X100mmol/LX0.002L = 74.278mg | ||
+ | |||
+ | ===June 15=== | ||
+ | |||
+ | Transformed the pTet and EYFP genes from the Biobrick registry | ||
+ | |||
+ | |||
+ | ===June 16=== | ||
+ | |||
+ | *Picked colonies in the early morning for Mini prep in the afternoon | ||
+ | |||
+ | *Restriction digested the plasmids: pTet with SpeI and PstI, EYFP with XbaI and PstI | ||
+ | |||
+ | ===June 17=== | ||
+ | |||
+ | *Quenched the restriction digests from the day before | ||
+ | |||
+ | ===June 18=== | ||
+ | |||
+ | *Checked the concentrations of: | ||
+ | **Riboswitch-1 : 4549u/.mL | ||
+ | **Riboswitch-2 : 4283ug/mL | ||
+ | **rpsA TIR-1 : 106ug/mL | ||
+ | **rpsA TIR-2 : 90ug/mL | ||
+ | **rpsA TIR-3 : 78ug/mL | ||
+ | **rpsA TIR-4 : 74ug/mL | ||
+ | **rpsA TIR-4b : 67ug/mL | ||
+ | **rpsA TIR-5 : 70ug/mL | ||
+ | |||
+ | in order to send for sequencing with the UR and UF2 primers | ||
+ | |||
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+ | .qmmc .qmdivider{display:block;font-size:1px;border-width:0px;border-style:solid;position:relative;z-index:1;}.qmmc .qmdividery{float:left;width:0px;}.qmmc .qmtitle{display:block;cursor:default;white-space:nowrap;position:relative;z-index:1;}.qmclear {font-size:1px;height:0px;width:0px;clear:left;line-height:0px;display:block;float:none !important;}.qmmc {position:relative;zoom:1;z-index:10;}.qmmc a, .qmmc li {float:left;display:block;white-space:nowrap;position:relative;z-index:1;}.qmmc div a, .qmmc ul a, .qmmc ul li {float:none;}.qmsh div a {float:left;}.qmmc div{visibility:hidden;position:absolute;}.qmmc .qmcbox{cursor:default;display:block;position:relative;z-index:1;}.qmmc .qmcbox a{display:inline;}.qmmc .qmcbox div{float:none;position:static;visibility:inherit;left:auto;}.qmmc li {z-index:auto;}.qmmc ul {left:-10000px;position:absolute;z-index:10;}.qmmc, .qmmc ul {list-style:none;padding:0px;margin:0px;}.qmmc li a {float:none;}.qmmc li:hover>ul{left:auto;}#qm0 ul {top:100%;}#qm0 ul li:hover>ul{top:0px;left:100%;} | ||
+ | |||
+ | |||
+ | /*!!!!!!!!!!! QuickMenu Styles [Please Modify!] !!!!!!!!!!!*/ | ||
+ | |||
+ | |||
+ | /* QuickMenu 0 */ | ||
+ | |||
+ | /*"""""""" (MAIN) Container""""""""*/ | ||
+ | #qm0 | ||
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+ | color:#3C13AF; | ||
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+ | |||
+ | |||
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+ | #qm0 .qmparent | ||
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+ | background-position:95% 50%; | ||
+ | } | ||
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+ | body #qm0 .qmactive, body #qm0 .qmactive:hover | ||
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+ | #qm0 div, #qm0 ul | ||
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+ | body #qm0 div .qmactive, body #qm0 div .qmactive:hover | ||
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+ | /*"""""""" Individual Horizontal Dividers""""""""*/ | ||
+ | #qm0 .qmdividerx | ||
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+ | margin:4px 5px 4px 5px; | ||
+ | border-color:#999999; | ||
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+ | |||
+ | /*"""""""" Custom Rule""""""""*/ | ||
+ | ul#qm0 ul | ||
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+ | |||
+ | /*"""""""" Custom Rule""""""""*/ | ||
+ | ul#qm0 li:hover > a.qmparent | ||
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+ | </style> | ||
+ | |||
+ | <!-- Add-On Core Code (Remove when not using any add-on's) --> | ||
+ | <style type="text/css">.qmfv{visibility:visible !important;}.qmfh{visibility:hidden !important;}</style><script type="text/javascript">if (!window.qmad){qmad=new Object();qmad.binit="";qmad.bvis="";qmad.bhide="";}</script> | ||
+ | |||
+ | <!-- Add-On Settings --> | ||
+ | <script type="text/JavaScript"> | ||
+ | |||
+ | /******* Menu 0 Add-On Settings *******/ | ||
+ | var a = qmad.qm0 = new Object(); | ||
+ | |||
+ | // Match Widths Add On | ||
+ | a.mwidths_active = true; | ||
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+ | a.overselects_active = true; | ||
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+ | </script> | ||
+ | |||
+ | <!-- Core QuickMenu Code --> | ||
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+ | |||
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+ | |||
+ | <!-- Add-On Code: IE Over Select Fix --> | ||
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+ | </head> | ||
+ | <body> | ||
+ | <ul id="qm0" class="qmmc"> | ||
+ | |||
+ | <li><a href="https://2009.igem.org/Team:Lethbridge">Home</a></li> | ||
+ | <li><a href="https://2009.igem.org/Team:Lethbridge/Notebook">Top of Page</a></li> | ||
+ | <li class="qmclear"> </li></ul> | ||
+ | |||
+ | <!-- Create Menu Settings: (Menu ID, Is Vertical, Show Timer, Hide Timer, On Click (options: 'all' * 'all-always-open' * 'main' * 'lev2'), Right to Left, Horizontal Subs, Flush Left, Flush Top) --> | ||
+ | <script type="text/javascript">qm_create(0,false,0,500,false,false,false,false,false);</script> | ||
+ | </body> | ||
+ | </html> | ||
+ | |||
+ | ===June 22=== | ||
+ | |||
+ | * Picked one colony each from DH5a + pTet and DH5a + EYFP. | ||
+ | *Grown overnight at 37 degrees in LB +100ug/mL Amp (5mL culture tubes) | ||
+ | *From mini-preps of EYFP(1&2) and pTet (1&2) did preparative restriction digests | ||
+ | **pTet with PstI and SpeI | ||
+ | **EYFP with XbaI and PstI | ||
+ | *In 37 degree water bath for 1hr and 20 min. Quenched at 60 degrees for 15 minutes. | ||
+ | |||
+ | ===June 23=== | ||
+ | |||
+ | *Ran a 1% agarose gel (1mL 50X TAE with 49mL Milli-Q H2O and 0.5g of agarose). | ||
+ | |||
+ | Lane 1: 1kb ladder | ||
+ | |||
+ | Lane 2:EYFP1A | ||
+ | |||
+ | Lane 3: EYFP1B | ||
+ | |||
+ | Lane 4: EYFP1B runover | ||
+ | |||
+ | Lane 5: EYFP2A | ||
+ | |||
+ | Lane 6: EYFP2B | ||
+ | |||
+ | Lane 7: pTet-1A | ||
+ | |||
+ | Lane 8: pTet-1B | ||
+ | |||
+ | Lane 9: pTet2-A | ||
+ | |||
+ | Lane 10: pTet-2B | ||
+ | |||
+ | *Samples were 2uL of dye and 10uL of DNA. | ||
+ | *The gel was unsuccessful. Possible reasons include: too short of an incubation during restriction digest or the enzymes were not functioning properly | ||
+ | |||
+ | [[Image:June_24_(June_23rd_work).JPG|250px]] | ||
+ | |||
+ | ===June 24=== | ||
+ | |||
+ | *Mini-Preps of pTet and EYFP | ||
+ | **750uL of culture from the fridge into microcentrifuge tubes. Pellet at 13000rpm for 2 min. Removed supernatant and added the rest of the culture. Repelleted at 13000rpm for 2 min. | ||
+ | **followed protocol according to Qiagen mini-prep protocol on page 2 | ||
+ | *Restriction Digest of EYFP and pTet | ||
+ | **EYFP restricted with XbaI and PstI | ||
+ | **pTet restricted with PstI and SpeI | ||
+ | ***Double digest:1uL buffer tango, 8uL DNA, 0.5uL of each enzyme | ||
+ | ***Single digest (1 for each enzyme): 0.5uL water, 1uLbuffer tango, 8uL DNA, 0.5uL enzyme | ||
+ | ***Negative control: 1uL water, 1uL buffer, 8uL DNA | ||
+ | ***8 tubes total in to the thermocycler for 8hrs at 37, 15min at 60 then held at 4 before going into the -20 fridge. | ||
+ | <html> | ||
+ | <head> | ||
+ | |||
+ | <!--%%%%%%%%%%%% QuickMenu Styles [Keep in head for full validation!] %%%%%%%%%%%--> | ||
+ | <style type="text/css"> | ||
+ | |||
+ | |||
+ | /*!!!!!!!!!!! QuickMenu Core CSS [Do Not Modify!] !!!!!!!!!!!!!*/ | ||
+ | .qmmc .qmdivider{display:block;font-size:1px;border-width:0px;border-style:solid;position:relative;z-index:1;}.qmmc .qmdividery{float:left;width:0px;}.qmmc .qmtitle{display:block;cursor:default;white-space:nowrap;position:relative;z-index:1;}.qmclear {font-size:1px;height:0px;width:0px;clear:left;line-height:0px;display:block;float:none !important;}.qmmc {position:relative;zoom:1;z-index:10;}.qmmc a, .qmmc li {float:left;display:block;white-space:nowrap;position:relative;z-index:1;}.qmmc div a, .qmmc ul a, .qmmc ul li {float:none;}.qmsh div a {float:left;}.qmmc div{visibility:hidden;position:absolute;}.qmmc .qmcbox{cursor:default;display:block;position:relative;z-index:1;}.qmmc .qmcbox a{display:inline;}.qmmc .qmcbox div{float:none;position:static;visibility:inherit;left:auto;}.qmmc li {z-index:auto;}.qmmc ul {left:-10000px;position:absolute;z-index:10;}.qmmc, .qmmc ul {list-style:none;padding:0px;margin:0px;}.qmmc li a {float:none;}.qmmc li:hover>ul{left:auto;}#qm0 ul {top:100%;}#qm0 ul li:hover>ul{top:0px;left:100%;} | ||
+ | |||
+ | |||
+ | /*!!!!!!!!!!! QuickMenu Styles [Please Modify!] !!!!!!!!!!!*/ | ||
+ | |||
+ | |||
+ | /* QuickMenu 0 */ | ||
+ | |||
+ | /*"""""""" (MAIN) Container""""""""*/ | ||
+ | #qm0 | ||
+ | { | ||
+ | width:auto; | ||
+ | background-color:transparent; | ||
+ | } | ||
+ | |||
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+ | </head> | ||
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+ | |||
+ | <li><a href="https://2009.igem.org/Team:Lethbridge">Home</a></li> | ||
+ | <li><a href="https://2009.igem.org/Team:Lethbridge/Notebook">Top of Page</a></li> | ||
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+ | |||
+ | ===June 25=== | ||
+ | |||
+ | *Ran a gel of the digested EYFP and pTet and controls from the previous day. | ||
+ | *Used 0.3g of agarose in 30mL of 1X TAE | ||
+ | *made stock solution of 1x TAE | ||
+ | *Ran gel at 100V for 1hr | ||
+ | |||
+ | Lane 1: 1kb ladder | ||
+ | |||
+ | Lane 2: Control-no enzyme(pTet) | ||
+ | |||
+ | Lane 3: pTet-pstI | ||
+ | |||
+ | Lane 4: pTet-SpeI | ||
+ | |||
+ | Lane 5: pTet-SpeI/PstI | ||
+ | |||
+ | Lane 6:EYFP-no enzyme | ||
+ | |||
+ | Lane 7: EYFP-PstI | ||
+ | |||
+ | Lane 8: EYFP-XbaI | ||
+ | |||
+ | Lane 9: EYFP-XbaI/PstI | ||
+ | |||
+ | Lane 10: 1kb ladder | ||
+ | |||
+ | *Gel melted | ||
+ | *Made 2 pTet and 2EYFP 5mL culture tubes with LB and Amp(100mg/mL). Left in incubator overnight at 37°C | ||
+ | |||
+ | ===June 26=== | ||
+ | |||
+ | *Cells harvested from pTet and EYFP cultures into 4 tubes. Spun down and LB supernatant removed. Stored in -20 for future use. | ||
+ | |||
+ | ===June 30=== | ||
+ | *200mL cultures of cells with pTet, EYFP and CFP grown in LB and 100ug/mL Amp harvested by centrifugation then maxi-prepped. | ||
+ | *Maxipreps | ||
+ | **incubated cell pellets in 3mL of ALSI and incubated at RT for 15min | ||
+ | **6mL of ASL2 added and incubated at RT for 10min | ||
+ | **4.5mL of AlS3 added and placed on ice for 10min | ||
+ | **Spun at 5000g at 4 for 15min | ||
+ | **5mL of each phenol and chloroform added to tubes containing resulting supernatant | ||
+ | **spun for 10min at 4 and 5000g, upper aqueous layer saved | ||
+ | **5mL of chloroform added to aqueous layer and spun for 10 min at 4 and 5000g. Supernatant saved | ||
+ | **0.6 volumes isopropanol added to each tube and placed in -20 freezer for 30min – | ||
+ | **spun for 10min at 4 and 5000g | ||
+ | **pellet wasted with EtOH and airdried overnight | ||
+ | |||
+ | *5 culture (500mL) flasks of LB made: 10g tryptone, 5g yeast extract, 10g salt and 1L water |
Revision as of 19:23, 21 October 2009
- Home
- Team
- Project
- Ethics
- Notebook
- Meetings
- Modeling
- Parts
- Collaboration
- Judging
- Extra Information on SynBio
Calendar
May
May 5
Roxanne, Megan, Alix, Mackenzie, Sebastian
- prepared Lb Media in test tubes -prepared 250mL LB agar for plates
- Prepared 500nM Tris-HCl (pH 8.0), EDTA (pH 8.0, 500nm) TE Buffer (pH 8.0), GTE (Solution I), 2M NaOH, 10% SDS
May 6
Roxanne
- Autoclaved LB test tubes, LB agar, Tris-HCl, EDTA, TE, GTE
- Added ampicillin to LB agar (100ug/mL) -Poured LB + amp plates
May 12
Roxanne
- Prepared LB agar
- added Tetracyclin (100ug/mL) –
- Poured LB + ampt plates
Roxanne, Alix, Ashley, Megan, Mackenzie, Kirsten
- transferred pE43 (DH5α) cells from gylcerol stock to 5mL LB+Tet test tube (x8)
- placed in orbital shaker overnight at 37°C
May 13
Roxanne
- Removed test tubes from shaker (16hrs incubation) and placed in deli fridge
May 14
Roxanne, Alix, Ashley, Mackenzie, Kirsten
- Preformed alkaline lysis miniprep on pE43 plasmid -lost plasmid from 2 tubes
- obtained 6X pE43 plasmid (2X ohbR, 2x ohbB, ohbA, ohbC)
May 19
Roxanne, Alix, Ashley, Kirsten, Megan, Mackenzie
- Gel Electrophoresis : 1% agarose in TAE
Lane 1: Ladder
Lane 2: ohbR1
Lane 3: ohbR2
Lane 4: ohbC
Lane 5: ohbB1
Lane 6: ohbB2
Lane 7:ohbA
Lane 8:ohbC
Lane 9: ohbB1
Lane 10:ohbB2
- DNA quantification by UV spec 260nm : 2.013 280nm: 1.105 260/280 : 1.984 Concentration: 2517µg/mL PCR of ohbA, (ohbB)x2, ohbC, (ohbR)x2
- Took picture of the gel - it did not turn out.
May 21
Roxanne
- Made 50X TAE Buffer
- Running PCR amplicons & RS/pSB1A2 ligation product on a 1% agarose gel
- Jeff gave tutorial on primer design and quick-change mutagenesis to Kirsten, Ashley, Mackenzie, Fan, Lisza, Roxanne
May 26
Roxanne, Alix, Megan, Mackenzie, Kirsten
- Gel did not turn out gave tutorial on open wetware and the igem registry
May 28
Roxanne
- reran the gel from may 19th, only primer dimers present
Roxanne, Ashley, Alix, Kirsten, Mackenzie, Megan
- Redoing the PCR of ohbA, ohbB, ohbC and OhbR with Phusion DNA Polymerase
Roxanne
- refilled the tip boxes
May 29
Roxanne
- prepared glycerol stocks for autoclaving
June
June 1
Roxanne
- Ran a 1% agarose in TAE gel of the PCR products from May 28th.
- 5µL of ladder, 2µL of DNA
Lane 1: ladder
Lane 2: ohbA (conc.1x)
Lane 3: ohbA (conc.1/10)
Lane 4: ohbB(1x)
Lane 5: ohbB(1/10)
Lane 6: ohbC(1x)
Lane 7: ohbC(1/10)
Lane 8: ohbR (1x)
Lane 9: ohbR(1/10)
Lane 10: ohbR(1x)
- Gel did not show any amplification
Mackenzie & Roxanne
- Transformation of pSB1A3 into DH5α
- Made 2 aliquots of pSB1A3 and 1 of pUC19
- plated pSB1A3-1: straight and dilute, pSB1A3-2: straight and dilute, pUC19: straight only incubated overnight at 37°C
June 3
Roxanne
- positive control worked
- Think the transformation worked but slight problem. The plasmid contains a suicide gene. Therefore, any cells that took up the plasmid would die.
- planning new genes to transform
- GENE LOCATION pSB1A3 + IPTG Inducible RFP 1-1k Bba_I13522, pTET GFP 2-8A Bba_I13521, pTet mRFP 2-6O Bba_I13600, pTET CFP 1-24E BBA-B0015, double terminator 1-23L
June 4
- Picked some glycerol stock GFP for the AIF visit
- made ampicillin plates 371.39g/mol X100mmol/LX0.002L = 74.278mg
June 15
Transformed the pTet and EYFP genes from the Biobrick registry
June 16
- Picked colonies in the early morning for Mini prep in the afternoon
- Restriction digested the plasmids: pTet with SpeI and PstI, EYFP with XbaI and PstI
June 17
- Quenched the restriction digests from the day before
June 18
- Checked the concentrations of:
- Riboswitch-1 : 4549u/.mL
- Riboswitch-2 : 4283ug/mL
- rpsA TIR-1 : 106ug/mL
- rpsA TIR-2 : 90ug/mL
- rpsA TIR-3 : 78ug/mL
- rpsA TIR-4 : 74ug/mL
- rpsA TIR-4b : 67ug/mL
- rpsA TIR-5 : 70ug/mL
in order to send for sequencing with the UR and UF2 primers
June 22
- Picked one colony each from DH5a + pTet and DH5a + EYFP.
- Grown overnight at 37 degrees in LB +100ug/mL Amp (5mL culture tubes)
- From mini-preps of EYFP(1&2) and pTet (1&2) did preparative restriction digests
- pTet with PstI and SpeI
- EYFP with XbaI and PstI
- In 37 degree water bath for 1hr and 20 min. Quenched at 60 degrees for 15 minutes.
June 23
- Ran a 1% agarose gel (1mL 50X TAE with 49mL Milli-Q H2O and 0.5g of agarose).
Lane 1: 1kb ladder
Lane 2:EYFP1A
Lane 3: EYFP1B
Lane 4: EYFP1B runover
Lane 5: EYFP2A
Lane 6: EYFP2B
Lane 7: pTet-1A
Lane 8: pTet-1B
Lane 9: pTet2-A
Lane 10: pTet-2B
- Samples were 2uL of dye and 10uL of DNA.
- The gel was unsuccessful. Possible reasons include: too short of an incubation during restriction digest or the enzymes were not functioning properly
June 24
- Mini-Preps of pTet and EYFP
- 750uL of culture from the fridge into microcentrifuge tubes. Pellet at 13000rpm for 2 min. Removed supernatant and added the rest of the culture. Repelleted at 13000rpm for 2 min.
- followed protocol according to Qiagen mini-prep protocol on page 2
- Restriction Digest of EYFP and pTet
- EYFP restricted with XbaI and PstI
- pTet restricted with PstI and SpeI
- Double digest:1uL buffer tango, 8uL DNA, 0.5uL of each enzyme
- Single digest (1 for each enzyme): 0.5uL water, 1uLbuffer tango, 8uL DNA, 0.5uL enzyme
- Negative control: 1uL water, 1uL buffer, 8uL DNA
- 8 tubes total in to the thermocycler for 8hrs at 37, 15min at 60 then held at 4 before going into the -20 fridge.
June 25
- Ran a gel of the digested EYFP and pTet and controls from the previous day.
- Used 0.3g of agarose in 30mL of 1X TAE
- made stock solution of 1x TAE
- Ran gel at 100V for 1hr
Lane 1: 1kb ladder
Lane 2: Control-no enzyme(pTet)
Lane 3: pTet-pstI
Lane 4: pTet-SpeI
Lane 5: pTet-SpeI/PstI
Lane 6:EYFP-no enzyme
Lane 7: EYFP-PstI
Lane 8: EYFP-XbaI
Lane 9: EYFP-XbaI/PstI
Lane 10: 1kb ladder
- Gel melted
- Made 2 pTet and 2EYFP 5mL culture tubes with LB and Amp(100mg/mL). Left in incubator overnight at 37°C
June 26
- Cells harvested from pTet and EYFP cultures into 4 tubes. Spun down and LB supernatant removed. Stored in -20 for future use.
June 30
- 200mL cultures of cells with pTet, EYFP and CFP grown in LB and 100ug/mL Amp harvested by centrifugation then maxi-prepped.
- Maxipreps
- incubated cell pellets in 3mL of ALSI and incubated at RT for 15min
- 6mL of ASL2 added and incubated at RT for 10min
- 4.5mL of AlS3 added and placed on ice for 10min
- Spun at 5000g at 4 for 15min
- 5mL of each phenol and chloroform added to tubes containing resulting supernatant
- spun for 10min at 4 and 5000g, upper aqueous layer saved
- 5mL of chloroform added to aqueous layer and spun for 10 min at 4 and 5000g. Supernatant saved
- 0.6 volumes isopropanol added to each tube and placed in -20 freezer for 30min –
- spun for 10min at 4 and 5000g
- pellet wasted with EtOH and airdried overnight
- 5 culture (500mL) flasks of LB made: 10g tryptone, 5g yeast extract, 10g salt and 1L water