Team:Heidelberg/Notebook/Killing I/Notebook/week3
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- | <a href="https://2008.igem.org/Team:Heidelberg/ | + | <a href="https://2008.igem.org/Team:Heidelberg/Modeling" style="color: white">Modeling<!--[if gt IE 6]><!--></a><!--<![endif]--> |
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- | <a href="https://2008.igem.org/Team:Heidelberg/Notebook/ | + | <a href="https://2008.igem.org/Team:Heidelberg/Notebook/Overview" style="color: white">Notebook<!--[if gt IE 6]><!--></a><!--<![endif]--> |
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<li style="width: 160px"> | <li style="width: 160px"> | ||
- | <a href="https://2008.igem.org/Team:Heidelberg/ | + | <a href="https://2008.igem.org/Team:Heidelberg/Human_Practice/Project_Overview" style="color: white">Human Practice<!--[if gt IE 6]><!--></a><!--<![endif]--> |
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<li><a href="https://2008.igem.org/Team:Heidelberg/Human_Practice/Surveys"><span><span>Surveys</span></span></a></li> | <li><a href="https://2008.igem.org/Team:Heidelberg/Human_Practice/Surveys"><span><span>Surveys</span></span></a></li> | ||
<li><a href="https://2008.igem.org/Team:Heidelberg/Human_Practice/Open_Day"><span><span>Open Day</span></span></a></li> | <li><a href="https://2008.igem.org/Team:Heidelberg/Human_Practice/Open_Day"><span><span>Open Day</span></span></a></li> | ||
- | <li><a href="https://2008.igem.org/Team:Heidelberg/Human_Practice/Nobel_Prize"><span><span>Nobel Prize</span></span></a></li> | + | <li><a href="https://2008.igem.org/Team:Heidelberg/Human_Practice/Nobel_Prize"><span><span>Nobel Prize</span></span></a></li> |
+ | |||
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+ | {| class="wikitable" | ||
+ | |- bgcolor=white | ||
+ | ! height=20px, width=250px | [[Team:Heidelberg/Notebook/Killing_I/Notebook/week2|<< Week 2]]|| width=500px | [[Team:Heidelberg/Notebook/Killing_I/Notebook|Overview]]|| width=250px | [[Team:Heidelberg/Notebook/Killing_I/Notebook/week4| Week 4 >> ]] | ||
+ | |-style="height:20px" | ||
+ | |} | ||
+ | |||
+ | '''Week 3''' | ||
==Monday, 08/18/08== | ==Monday, 08/18/08== | ||
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** Analytical digestion of cI "green", cI "black" and T9002 | ** Analytical digestion of cI "green", cI "black" and T9002 | ||
- | *Gel | + | *Gel |
- | + | [[Image:Hd-phage-08-08-19-digestion.jpg]] | |
#* Lane 0: DNA ladder mix | #* Lane 0: DNA ladder mix | ||
#* Lane 1: lambda DNA | #* Lane 1: lambda DNA | ||
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** --> cI does not work!!!! | ** --> cI does not work!!!! | ||
*growing curve | *growing curve | ||
- | + | [[Image:Hd-phage-wachstumskurve_errorbars_small.jpg]] | |
**the values are the average of all four cultures | **the values are the average of all four cultures | ||
- | + | ||
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===project planning=== | ===project planning=== | ||
- | Guys, we received this email by another professor in the states. sounds good. we should get this helper plasmids in the end :) | + | Guys, we received this email by another professor in the states. sounds good. we should get this helper plasmids in the end :) |
- | + | ||
I have sent pUB307, RSF1010, pED350, pED361, which are described in our two MGG papers. Also two clones I made of the oriT from RP1; pED369 and pED374. There are 10microl of each. The DNAs are old (1983!) and so I would transform and make | I have sent pUB307, RSF1010, pED350, pED361, which are described in our two MGG papers. Also two clones I made of the oriT from RP1; pED369 and pED374. There are 10microl of each. The DNAs are old (1983!) and so I would transform and make | ||
fresh plasmid preps. | fresh plasmid preps. | ||
- | + | ||
pED350 is oriT+ and Mob+, so it is efficiently mobilised by RPI or its derivative pUB307. pED361 is oriT+ only. It cannot be mobilised by pUB307 as it lacks mob functions. If RSF1010 is also in the cell pKD361 is very efficiently mobilised by pUB307. | pED350 is oriT+ and Mob+, so it is efficiently mobilised by RPI or its derivative pUB307. pED361 is oriT+ only. It cannot be mobilised by pUB307 as it lacks mob functions. If RSF1010 is also in the cell pKD361 is very efficiently mobilised by pUB307. | ||
- | + | ||
pED369 and pED374 are two subclones I made of the RP1 oriT into pED825 (Amp resistant described in MGG papers). pED374 contains a single 690 bp HaeII fragment containing the | pED369 and pED374 are two subclones I made of the RP1 oriT into pED825 (Amp resistant described in MGG papers). pED374 contains a single 690 bp HaeII fragment containing the | ||
RP1 oriT. PED369 contains the 690 bp oriT fragment plus additional HaeII fragments. I sent both just in case the pED374 DNA does not check out. These are efficiently | RP1 oriT. PED369 contains the 690 bp oriT fragment plus additional HaeII fragments. I sent both just in case the pED374 DNA does not check out. These are efficiently | ||
mobilised by pUB307. | mobilised by pUB307. | ||
- | + | ||
I would think cloning this 690 bp fragment into your lambda vector would be the simplest | I would think cloning this 690 bp fragment into your lambda vector would be the simplest | ||
solution; its small and will mobilise in the presence of just pUB307. | solution; its small and will mobilise in the presence of just pUB307. | ||
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Keith | Keith | ||
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<hr> | <hr> | ||
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==Wednesday, 08/20/08== | ==Wednesday, 08/20/08== | ||
Line 277: | Line 614: | ||
*Gel | *Gel | ||
- | + | [[Image:Hd-phage-08-08-20-digestion.jpg]] | |
* Lane 0: DNA ladder mix | * Lane 0: DNA ladder mix | ||
Line 297: | Line 634: | ||
- | ===overview of the | + | ===overview of the phage cloning strategy one=== |
<br> | <br> | ||
- | + | [[Image:Hd-phage-Klonierungsstrategie_Page_1.jpg]] | |
<br><br><br> | <br><br><br> | ||
- | + | [[Image:Hd-phage-Klonierungsstrategie_Page_2.jpg]] | |
<br><br><br><br><br><br> | <br><br><br><br><br><br> | ||
- | + | [[Image:Hd-phage-Klonierungsstrategie_Page_3.jpg]] | |
<br><br><br> | <br><br><br> | ||
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<br><br><br> | <br><br><br> | ||
Used primer sequences: | Used primer sequences: | ||
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oriT_RP4_fw (Tm=62°C): | oriT_RP4_fw (Tm=62°C): | ||
Line 316: | Line 652: | ||
CTCGTTTCTAGAACTAGTgacaggctcatgccggccgc | CTCGTTTCTAGAACTAGTgacaggctcatgccggccgc | ||
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oriT_RP4_rv: (Tm=58°C) | oriT_RP4_rv: (Tm=58°C) | ||
TATTCGGGTACCgtcccctcagttcagtaatttcctgc | TATTCGGGTACCgtcccctcagttcagtaatttcctgc | ||
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GFP_CmR_fw: (Tm=56°C) | GFP_CmR_fw: (Tm=56°C) | ||
CTCGTTGGTACCTCTAGAtttacagctagctcagtcctagg | CTCGTTGGTACCTCTAGAtttacagctagctcagtcctagg | ||
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GFP_CmR_rv: (Tm=55°C) | GFP_CmR_rv: (Tm=55°C) | ||
TATTCGACCGGTACTAGTtataaacgcagaaaggcccacc | TATTCGACCGGTACTAGTtataaacgcagaaaggcccacc | ||
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GAM_fw: (Tm=55°C) | GAM_fw: (Tm=55°C) | ||
AGTGCTTTAGCGTTAACTTCCG | AGTGCTTTAGCGTTAACTTCCG | ||
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GAM_rv: (Tm=53°C) | GAM_rv: (Tm=53°C) | ||
GGTTTTACCGCATACCAATAACG | GGTTTTACCGCATACCAATAACG | ||
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CmR_fw: (Tm=54°C) | CmR_fw: (Tm=54°C) | ||
gctaaaATGgagaaaaaaatcactgg | gctaaaATGgagaaaaaaatcactgg | ||
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CmR_rv: (Tm=58°C) | CmR_rv: (Tm=58°C) | ||
AGGTTCTCCTTTATTAGCCGGATCCTCTAGATTACGCC | AGGTTCTCCTTTATTAGCCGGATCCTCTAGATTACGCC | ||
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==Thursday, 08/21/08== | ==Thursday, 08/21/08== | ||
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* Gel | * Gel | ||
- | + | [[Image:Hd-phage-08-08-21-lambda.jpg]] | |
** lane 0: DNA ladder mix | ** lane 0: DNA ladder mix | ||
** lane 2: lambda DNA (fermentas) (XbaI, XhoI --> ~40 kb, ~9 kb) | ** lane 2: lambda DNA (fermentas) (XbaI, XhoI --> ~40 kb, ~9 kb) | ||
Line 423: | Line 754: | ||
* Gel | * Gel | ||
- | + | [[Image:Hd-phage-08-08-21-digestion_I20260.jpg]] | |
*** lane 0: DNA ladder | *** lane 0: DNA ladder | ||
*** lane 1: I20260 1 | *** lane 1: I20260 1 | ||
Line 455: | Line 786: | ||
* Gel: Digestions of lambda-DNA (fermentas), and the small XbaI-XhoI fragments | * Gel: Digestions of lambda-DNA (fermentas), and the small XbaI-XhoI fragments | ||
- | + | [[Image:Hd-phage-08-08-22-digestion.jpg]] | |
** lane 1: DNA ladder mix | ** lane 1: DNA ladder mix | ||
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** large fragment 1: 14,4 ng/µl; 1,99 | ** large fragment 1: 14,4 ng/µl; 1,99 | ||
** large fragment 1: 16,8 ng/µl; 2,14 | ** large fragment 1: 16,8 ng/µl; 2,14 | ||
+ | |||
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+ | {| class="wikitable" | ||
+ | |- bgcolor=white | ||
+ | ! height=20px, width=250px | [[Team:Heidelberg/Notebook/Killing_I/Notebook/week2|<< Week 2]]|| width=500px | [[Team:Heidelberg/Notebook/Killing_I/Notebook|Overview]]|| width=250px | [[Team:Heidelberg/Notebook/Killing_I/Notebook/week4| Week 4 >> ]] | ||
+ | |-style="height:20px" | ||
+ | |} |
Latest revision as of 11:34, 29 October 2008
<< Week 2 | Overview | Week 4 >> |
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Week 3
Contents |
Monday, 08/18/08
chloramphenicol resistance cassette
- Maxiprep of P1000, P1004, B0014, B0015
- P1000 1672 ng/µl 1,92
- P1004 1153 ng/µl 1,92
- B0014 2040,4 ng/µl 1,92
- B0015 1053,6 ng/µl 1,92
- Analytical digestions
- lambda DNA with XbaI and XhoI
2µl DNA 5µl NEB2 5µl BSA 1µl XbaI 1µl XhoI 26µl water
- Analytical digestion of P1000
1µl DNA 2µl NEB3 2µl NcoI 15µl water
- Analytical digestion of P1004
1µl DNA 2µl NEB4 1,5µl DraI 15,5µl water
- Analytical digestion of B0014 / B0015
1µl DNA 2µl NEB4 2µl BSA 2,5µl SfcI 12,5µl water
- Analytical digestion of cI "green", cI "black" and T9002
- Gel
- Lane 0: DNA ladder mix
- Lane 1: lambda DNA
- Lane 2: lambda DNA (XbaI, XhoI --> large frament ~ 40kb, small fragment ~ 9kb)
- Lane 3: P1000
- Lane 4: P1000 (NcoI-->1473,2374)
- Lane 5: P1004
- Lane 6: P1004 (DraI-->19,339,692,1067,1360)
- Lane 7: cI green
- Lane 8: cI green (NdeI - expected fragments?)
- Lane 9: cI black
- Lane 10: cI black (NdeI)
- Lane 11: T9002
- Lane 12: T9002 (NdeI - expected fragments?)
lamda phage
Infectiontest
- inoculation of 20ml medium with over night culture (MG1655)
- after 1h plaque added --> 37C for 2h + inoculation of ZMBH phage (100ql 10^-2 in 20ml MG1655)
- incubation at 42C for 2 more hours
- sterilefiltration + mix with growing bacteria (MG1655 and MG1655+cI)
- incubate in soft agar at 37C for 2h, than at 42C for another 4h (altogether 24 plates)
- phage DNA was also isolated from filtrate
- results:
- same amount of plaques on plates with MG1655 as with MG1655+cI
- nearly no plaques on plates with own phage --> very low phage concentration
- --> cI does not work!!!!
- growing curve
- the values are the average of all four cultures
Tuesday, 08/19/08
lambda phage
- Digestion of lambda DNA with XbaI and XhoI
- very nice separation of the small fragment from the two large fragments (one band) picture of the gel was not saved but it looked very nice
- cutting out of the small and large fragment --> gel purification kit
- small fragment: 30,3 ng/µl; 1,86
- large fragment1: 19,5 ng/µl; 2,11
- large fragment2: 61,5ng/µl; 1,90
GFP
- inoculation of three overnight cultures from the two I20260 glycerol stocks
chloramphenicol resistance cassette
- Transformation of P1000, P1004 (both chloramphenicol resistances) and CI
- no success
project planning
Guys, we received this email by another professor in the states. sounds good. we should get this helper plasmids in the end :)
I have sent pUB307, RSF1010, pED350, pED361, which are described in our two MGG papers. Also two clones I made of the oriT from RP1; pED369 and pED374. There are 10microl of each. The DNAs are old (1983!) and so I would transform and make fresh plasmid preps.
pED350 is oriT+ and Mob+, so it is efficiently mobilised by RPI or its derivative pUB307. pED361 is oriT+ only. It cannot be mobilised by pUB307 as it lacks mob functions. If RSF1010 is also in the cell pKD361 is very efficiently mobilised by pUB307.
pED369 and pED374 are two subclones I made of the RP1 oriT into pED825 (Amp resistant described in MGG papers). pED374 contains a single 690 bp HaeII fragment containing the RP1 oriT. PED369 contains the 690 bp oriT fragment plus additional HaeII fragments. I sent both just in case the pED374 DNA does not check out. These are efficiently mobilised by pUB307.
I would think cloning this 690 bp fragment into your lambda vector would be the simplest solution; its small and will mobilise in the presence of just pUB307.
Keith
Wednesday, 08/20/08
GFP
- Miniprep of reference promotor I20260
- Concentrations:
- Epi1 9,8 ng/ul; 2,52
- Epi2 15,7 ng/ul; 2,28
- Epi3 19,7 ng/ul; 1,93
- Concentrations:
- Digestion of I20260
10 µl DNA (from Epi3) 2ul SmlI 12µl NEB4 2ul BSA 10x 4 µl water
- Digestion of the XbaI-XhoI fragment with AgeI
18 µl DNA (from gel purification kit) 5 µl AgeI 5 µl NEB4 22 µl water
- Gel
- Lane 0: DNA ladder mix
- Lane 1: I20260 (SmlI-->251bp, 373bp, 843bp, 918bp, 1284bp)
- Lane 2: XbaI-XhoI fragment (AgeI-->1.7kb, 7.3kb)
- Lane 3: large lambda DNA fragments 3µl (15kb, 24.5kb)
- Results:
- I20260 seems not to be correct, inoculate overnight cultures from the glycerol stocks again
- digestion of the XbaI-XhoI fragment with AgeI did not work good, only the 7.3kb fragment can be seen, reasons: wrong buffer concentration, too much enzyme (glycerol) in the reaction
- large lambda DNA fragment is looking good
lambda phage
- concentrations of lambda-DNA extractions
- from Fermentas Phage - plaque 1: 7.5 ng/ul; 1.86
- from Fermentas Phage - plaque 2: 61.5 ng/ul 1.90
- from ZMBH phage 19,7 ng/ul 2,11
overview of the phage cloning strategy one
Used primer sequences:
oriT_RP4_fw (Tm=62°C):
CTCGTTTCTAGAACTAGTgacaggctcatgccggccgc
oriT_RP4_rv: (Tm=58°C)
TATTCGGGTACCgtcccctcagttcagtaatttcctgc
GFP_CmR_fw: (Tm=56°C)
CTCGTTGGTACCTCTAGAtttacagctagctcagtcctagg
GFP_CmR_rv: (Tm=55°C)
TATTCGACCGGTACTAGTtataaacgcagaaaggcccacc
GAM_fw: (Tm=55°C)
AGTGCTTTAGCGTTAACTTCCG
GAM_rv: (Tm=53°C)
GGTTTTACCGCATACCAATAACG
CmR_fw: (Tm=54°C)
gctaaaATGgagaaaaaaatcactgg
CmR_rv: (Tm=58°C)
AGGTTCTCCTTTATTAGCCGGATCCTCTAGATTACGCC
Thursday, 08/21/08
lambda phae
- Preparative digestion of lambda-DNA from Fermentas
10µl DNA = 3 ug 2µl XhoI 2µl XbaI 5µl NEB 2 5µl BSA 33µl H20
- lambda DNA "2" and "ZMBH" from phage extraction kit
36 µl DNA 2 µl XhoI 2µl XbaI 5µl NEB 2 5 µl BSA
- all digestions 3h, 400rpm, 37°
- Gel
- lane 0: DNA ladder mix
- lane 2: lambda DNA (fermentas) (XbaI, XhoI --> ~40 kb, ~9 kb)
- lane 4: lambda DNA from extraction "2" (XbaI, XhoI --> ~40 kb, ~9 kb)
- lane 6: lambda DNA from extraction "ZMBH phage" (XbaI, XhoI --> ~40 kb, ~9 kb)
- lane 2, 4 and 6 overflowed
- cutting out of the XbaI-XhoI fragment from lane 2
- the large fragment wasn't cutted out because the gel was exposed to UV light over 30 seconds
- gel extraction kit
- DNA eluted in 20µl
- Digestion of the XbaI-XhoI fragment with AgeI
20µl DNA (from gel purification kit) 2µl AgeI 5µl NEB4 23µl water
- 16°C over night
- Preparative digestion of lambda-DNA from Fermentas
10µl DNA = 3 µg 2µl XhoI 2µl XbaI 5µl NEB 2 5µl BSA 33µl water
- 16°C over night
GFP
- Miniprep from overnight cultures of I20260 glycerol stocks
- eluted in 50 µl
- Concentrations:
- Miniprep 1: 19.8 ng/µl
- Miniprep 2: 17.4 ng/µl
- Miniprep 3: 19.0 ng/µl
- Miniprep 4: 16.4 ng/µl
- Analytical digestion of the four I20260 Minipreps
- 20µl DNA
- 5µl NEB 4
- 1.5µl DraI
- 23.5µl water
- Gel
- lane 0: DNA ladder
- lane 1: I20260 1
- lane 2: I20260 1 (DraI-->19bp, 535bp, 886bp, 2229bp)
- lane 3: I20260 2
- lane 4: I20260 2 (DraI)
- lane 5: I20260 3
- lane 6: I20260 3 (DraI)
- lane 7: I20260 4 (DraI)
- Results
- it seems that we have I20260, inoculation of an overnight culture from I2020 No. 3 for Maxiprep
- Results
- Transformation of I20260 (Kan) (from the promotor measurement kit sheet as well as from the registry) and J01101 (Amp)
- eluted in 10µl water
- transformed into TOP10 and MG1655 (each 4µl DNA)
cI
- ordered J01101 (cI) from the iGEM headquater, they will already send it today
Friday, 08/22/08
GFP
- Maxiprep of reference promotor I20260
- concentrations: 200 ng/µl
lambda phage
- Gel: Digestions of lambda-DNA (fermentas), and the small XbaI-XhoI fragments
- lane 1: DNA ladder mix
- lane 3: lambda-DNA (XbaI, XhoI; ~ 40kb, ~ 9kb)
- lane 5: small lambda-fragment assayI (AgeI, ~1,7kb, ~7,3kb)
- lane 7: small lambda-fragment assayII (AgeI, ~1,7kb, ~7,3kb)
- Extraction of XbaI-XhoI fragments (evaluation of samples with nanodrop)
- small fragment 1: 15,9 ng/µl; 2,41
- small fragment 2: 6,6 ng/µl; 2,02
- large fragment 1: 14,1 ng/µl; 2,75
- large fragment 1: 10,8 ng/µl; 2,86
- large fragment 1: 14,4 ng/µl; 1,99
- large fragment 1: 16,8 ng/µl; 2,14
<< Week 2 | Overview | Week 4 >> |
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