Difference between revisions of "Part:BBa K1463000"
 
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<partinfo>BBa_K1463000 short</partinfo>
 
<partinfo>BBa_K1463000 short</partinfo>
  
A recombinase switch with GFP one side of the switch and RFP on the other.
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A recombinase switch with GFP one side of the switch and RFP on the other.<br>
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PhiC31 integrase flips the orientation of the DNA between attP and attB, changing the direction of the promoter, switching rfp off and gfp on.
  
[[Image:GU_jake_gel_1.jpg‎|thumb|500px|right|'''Fig. 1:''' BL21 ''E. coli'' carrying different constructs on [http://2012.igem.org/Team:Goettingen/Project/Materials#M9_Swimming_Agar M9 minimal medium swarming agar]. after 48h incubation at 33°C. Cells expressing ''fliC'' in puc18 under the natural promoter travelled approximately 1,5cm (radius) whereas no swimming could be detected for the control plasmid carrying [https://parts.igem.org/Part:BBa_K777125 K777125]. On tryptone swimming agar ''yhjH'' transformants were usually faster.]]
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[[Image:switchint.png|thumb|center|600px|'''Fig. 1:''' Diagram of the BBa_K1463000 recombination switch. ]]
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===Usage and Biology===
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Recombination was tested in vivo by placing BBa_K1463000 on a low copy number pSC101 plasmid and introducing a second plasmid (pBAD-int) that only expresses integrase when arabinose is added.
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[[Image:Switchgelann.jpg|thumb|center|500px|'''Fig. 2:''' In vivo recombination of BBa_K1463000 switch using a plasmid (pBAD-Int) that expresses PhiC31 integrase under the control of the arabinose inducible Pbad promoter. Cells were grown for 16 hours with arabinose or glucose. Plasmid DNA was purified, cut with BamHI, which cuts once in the switch and once in the vector, and run on a 1.2% agarose gel.The gel shows three replicates of the same experiment. 1.pBAD-Int on its own, 2.Switch #2 on its own, 3.Switch #2 + pBAD-Int glucose, 4.Switch #2 + pBAD-Int arabinose, 5.Switch #3 on its own, 6.Switch #3 + pBAD-Int glucose, 7.Switch #3 + pBAD-Int arabinose, 8.Switch #4 on its own, 9.Switch #4 + pBAD-Int glucose, 10.Switch #4 + pBAD-Int arabinose, 11.pBAD33 gvpAC (ignore)12.1kb+ marker.]]
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The BamHI sites are placed in such a way that the bands produced by digestion with this restriction enzyme change depending on whether recombination has occurred or not. This pattern can be seen on the gel above.
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Sizes of fragments using BamHI are:
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RFP ON GFP OFF (attP and attB) 2339 bp + 2776 bp
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GFP ON RFP OFF (attL and attR) 2477 bp + 2628 bp
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As can be seen, the restriction pattern changes from RFP ON to GFP ON only when arabinose is added.
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[[Image:Fluoann1.jpg|thumb|center|800px|'''Fig. 3:''' Fluorescence scan showing RFP and GFP fluorescence when BBa_K1463000 recombination switch is grown in vivo with pBAD-int with glucose or arabinose. 200 ul samples of overnight cultures in a 96 well plate scanned using a Typhoon FLA9500 scanner. Overlay of red and green fluorescent images using 532 nm laser and LPG filter and 473 laser and BPB filter respectively. Samples in the middle two rows are duplicate samples of cells corresponding to lanes 3, 4, 6, 7, 9, 10, 2, 5, 8 and 11 in the gel in Fig 2 above. That is the first 6 wells from left to right contain the switch plus pBAD-int treated alternatively with glucose and arabinose, followed by three wells with just switch plasmid on its own (unswitched RFP ON), and a negative control with no RFP or GFP genes.]]
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There is a corresponding switch from red fluorescence to green fluorescence as the orientation of the promoter segment changes under the influence of integrase (Fig. 3).
  
[[Image:GU_jake_gel_1.jpg‎|thumb|center|500px|Calibration curve of concentration of GFP against fluorescence. The conversion factor is 79.429.]]
 
  
  
  
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===Usage and Biology===
 
  
 
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Latest revision as of 16:41, 17 October 2014

Recombinase Switch With GFP and RFP

A recombinase switch with GFP one side of the switch and RFP on the other.
PhiC31 integrase flips the orientation of the DNA between attP and attB, changing the direction of the promoter, switching rfp off and gfp on.

Fig. 1: Diagram of the BBa_K1463000 recombination switch.

Usage and Biology

Recombination was tested in vivo by placing BBa_K1463000 on a low copy number pSC101 plasmid and introducing a second plasmid (pBAD-int) that only expresses integrase when arabinose is added.

Fig. 2: In vivo recombination of BBa_K1463000 switch using a plasmid (pBAD-Int) that expresses PhiC31 integrase under the control of the arabinose inducible Pbad promoter. Cells were grown for 16 hours with arabinose or glucose. Plasmid DNA was purified, cut with BamHI, which cuts once in the switch and once in the vector, and run on a 1.2% agarose gel.The gel shows three replicates of the same experiment. 1.pBAD-Int on its own, 2.Switch #2 on its own, 3.Switch #2 + pBAD-Int glucose, 4.Switch #2 + pBAD-Int arabinose, 5.Switch #3 on its own, 6.Switch #3 + pBAD-Int glucose, 7.Switch #3 + pBAD-Int arabinose, 8.Switch #4 on its own, 9.Switch #4 + pBAD-Int glucose, 10.Switch #4 + pBAD-Int arabinose, 11.pBAD33 gvpAC (ignore)12.1kb+ marker.


The BamHI sites are placed in such a way that the bands produced by digestion with this restriction enzyme change depending on whether recombination has occurred or not. This pattern can be seen on the gel above.

Sizes of fragments using BamHI are:

RFP ON GFP OFF (attP and attB) 2339 bp + 2776 bp

GFP ON RFP OFF (attL and attR) 2477 bp + 2628 bp

As can be seen, the restriction pattern changes from RFP ON to GFP ON only when arabinose is added.


Fig. 3: Fluorescence scan showing RFP and GFP fluorescence when BBa_K1463000 recombination switch is grown in vivo with pBAD-int with glucose or arabinose. 200 ul samples of overnight cultures in a 96 well plate scanned using a Typhoon FLA9500 scanner. Overlay of red and green fluorescent images using 532 nm laser and LPG filter and 473 laser and BPB filter respectively. Samples in the middle two rows are duplicate samples of cells corresponding to lanes 3, 4, 6, 7, 9, 10, 2, 5, 8 and 11 in the gel in Fig 2 above. That is the first 6 wells from left to right contain the switch plus pBAD-int treated alternatively with glucose and arabinose, followed by three wells with just switch plasmid on its own (unswitched RFP ON), and a negative control with no RFP or GFP genes.

There is a corresponding switch from red fluorescence to green fluorescence as the orientation of the promoter segment changes under the influence of integrase (Fig. 3).



Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    INCOMPATIBLE WITH RFC[12]
    Illegal NheI site found at 813
    Illegal NheI site found at 836
  • 21
    INCOMPATIBLE WITH RFC[21]
    Illegal BamHI site found at 793
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    INCOMPATIBLE WITH RFC[25]
    Illegal AgeI site found at 34
    Illegal AgeI site found at 146
  • 1000
    INCOMPATIBLE WITH RFC[1000]
    Illegal BsaI.rc site found at 711
    Illegal BsaI.rc site found at 1668