Team:Freiburg/Notebook/27 July

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<a href="https://2011.igem.org/Team:Freiburg/Notebook/26_July">Previous entry</a>
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<a href="https://2011.igem.org/Team:Freiburg/Notebook"> 27 July </a>
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==Commons==
==Commons==
===Gel===
===Gel===
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We loaded the PCR products of the vectors on a gel and measured the DNA concentration.
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'''Investigators: Sandra, Sophie'''
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We loaded the PCR products of the vectors on a gel and measured the DNA concentration. DNA concentration were high and we diluted the vectors to get an endconcentration of 25ng/microl.
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'''Investigators: Sandra, Sophie'''
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'''DNA-concentration measured with nanodrop:'''<br/>
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{|cellpadding="10" cellspacing="0" border="1"
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|sample
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|DNA concentration (ng/μl)
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|-
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|pSB1C3
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|132.1
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|-
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|pSB1K3
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|101.5
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|-
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|pSB1A3
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|83.9
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|-
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|pSB1T3
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|116.2
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|}
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[[File:.Gelbild_Vektoren_27_07.jpg|350px|caption]]
==<span style="color:green;">green light receptor</span>==
==<span style="color:green;">green light receptor</span>==
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===NAME OF YOUR EXPERIMENT===
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===Results of Sequencing===
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'''Investigators:Julia'''
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CcaS 4a2 seemed to miss about 20bp, CcaS 4b2 is correct.
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===Quickchange PCR of CcaS and CcaR===
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'''Investigators:Julia'''
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in order to eliminate iGEM restriction sites of EcoRI within CcaS and CcaR, we designed mutagenesis primer and performed a quickchange PCR.
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===Protocol===
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total reaction volume is 50µl:
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32,5 µl H2O<br/>
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10 µl Phusion Buffer 5x<br/>
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2,5 µl Primer up<br/>
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2,5 µl Primer dw<br/>
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1 µl DNA template, concentration has to be 5ng/µl<br/>
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0,5 µl Phusion<br/>
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'''Investigators:NAME'''
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Primer for CcaR:<br/>
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ccaR_mut1_up: CCtcactaATGAGgATcCTTTTAGTGGAGG<br/>
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ccaR_mut1_dw:CCTCCACTAAAAGgATcCTCATtagtgaGG<br/>
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<br/>
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Primer for CcaS:<br/>
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ccaS_mut1_up:CCGGGCCGAGgATcCTCTATGTCAATG<br/>
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ccaS_mut1_dw:CATTGACATAGAGgATcCTCGGCCCGG<br/>
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<br/>
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Primer for CcaS:<br/>
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ccaS_mut2_up:GGACCAAAAACgAGTCGCACTGAATTAG<br/>
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ccaS_mut2_dw:CTAATTCAGTGCGACTcGTTTTTGGTCC<br/>
==<span style="color:blue;">blue light receptor</span>==
==<span style="color:blue;">blue light receptor</span>==
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We repeated the PCR again, with higher temperatures this time.
We repeated the PCR again, with higher temperatures this time.
After PCR we digested with DpnI 37°C for 1 hour and then purified the DNA with PCR purifictaion kit. Afterwards we measured the DNA concentration and loaded 2 microl to a gel.
After PCR we digested with DpnI 37°C for 1 hour and then purified the DNA with PCR purifictaion kit. Afterwards we measured the DNA concentration and loaded 2 microl to a gel.
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'''PCR'''
'''PCR'''
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|-
|-
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| colspan="2"  style="border:0.0069in solid #00000a;padding-top:0in;padding-bottom:0in;padding-left:0.075in;padding-right:0.075in;"| Continue from Experiment: NOT-Gate and LovTAP with Gibson-overhangs (now we use a little bit higher temperature for primer annealing) (Date): 25.07.11
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| colspan="2"  style="border:0.0069in solid #00000a;padding-top:0in;padding-bottom:0in;padding-left:0.075in;padding-right:0.075in;"| Continue from Experiment: NOT-Gate and LovTAP with Gibson-overhangs (now we use a little bit higher temperature for primer annealing) -(Date): 25.07.11
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(Name): Blue Light
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(Name): Sandra, Sophie
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|-
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| colspan="2"  style="border:0.0069in solid #00000a;padding-top:0in;padding-bottom:0in;padding-left:0.075in;padding-right:0.075in;"| Project Name:
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| colspan="2"  style="border:0.0069in solid #00000a;padding-top:0in;padding-bottom:0in;padding-left:0.075in;padding-right:0.075in;"| Project Name: Blue Light
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|}
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What program do you use?
What program do you use?
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57c auf 70c (in reality: 58c and then 68c)
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"57°C auf 70°C" (first annealing temperature: 58°C and then after 10 cycles 68°C)
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How did you label the PCR-Product, where is it stored and what do you do next?
How did you label the PCR-Product, where is it stored and what do you do next?
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==<span style="color:red;">red light receptor</span>==
 
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===NAME OF YOUR EXPERIMENT===
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'''DNA-concentration measured with nanodrop:'''
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'''Investigators:NAME'''
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{| cellpadding="10" cellspacing="0" border="1"
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|sample
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|DNA-concentration (ng/μl)
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|-
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|S35
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|75.1
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|-
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|S45
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|45.1
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|}
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==<span style="color:grey;">Precipitator</span>==
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==<span style="color:orange;">Lysis cassette</span>==
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Ruediger  27.07
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picked colonies from yesterdays Trafo into medium with 2μl/ml Tet
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===NAME OF YOUR EXPERIMENT===
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S39-P18
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S39-P19
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'''Investigators:NAME'''
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S39-P20
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==<span style="color:grey;">Precipitator</span>==
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===NAME OF YOUR EXPERIMENT===
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S43-P18
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S43-P19
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S43-P20
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'''Investigators: NAME'''
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overnight in 37°C

Latest revision as of 01:01, 22 September 2011


This is the wiki page
of the Freiburger student
team competing for iGEM 2011.
Thank you for your interest!