Difference between revisions of "Part:BBa K2120201"

 
 
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<partinfo>BBa_K2120201 short</partinfo>
 
<partinfo>BBa_K2120201 short</partinfo>
  
tetR repressible promoter. The function is similar with pTet[Part:BBa_R0040]. We mutated the -35 region and selected one with lower strength.It can be used to control the expression of toxin proteins to avoid leaking out.  
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tetR repressible promoter. The function is similar with pTet [https://parts.igem.org/wiki/index.php?title=Part:BBa_R0040  BBa_R0040]. We mutated the -35 region and selected one with lower strength.It can be used to control the expression of toxin proteins to avoid leaking out.  
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===A series of Ptet promoters===
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We designed a killer switch controlled by TetR repressor. When the concentration of inhibitors reduces to a threshold, the downstream in-promoter Ptet will start the transcription of killer gene. After measuring the original promoter strength [Part:BBa_R0040], we found that the activity is too high to be well controlled for expressing killer genes. So we mutated the original promoter and got 4 mutants with lower activity.
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'''Design'''
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We analyzed the promoter region and decided to mutated the -35 region through designing random primers. It can at most ensure the change of promoter’s background activity and maintain the promoter’s character since the tightly binding region with repressor is well-conserved while the tightly binding region with RNA polymerase is changed .
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'''Characterization using RFP'''
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The four mutated promoters were characterized using RFP to measure the level of gene expression. Cells were grown in 1.5 mL tube in LB culture medium. The host we used is E.coli TOP10.
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'''Results'''
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Cells showed Red fluorescence under fluorescence microscopy. Quantitative measurement was carried out through enzyme-labeled instrument. It turned out that the highest activity of mutants is about 500, while the common activity is about 200. The original promoter is 9000.
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[[File:BIT-CHINA-PARTS-MUTATION-1.jpg|600px|thumb|center|Fig1. Compared with the original promoter, the promoter strength of mutants Ptet-1, Ptet-2, Ptet-3, Ptet-25 is sharply decreased.]]
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We have submitted four mutated promoters [[https://parts.igem.org/wiki/index.php?title=Part:BBa_K2120200  BBa_K2120200]; [https://parts.igem.org/wiki/index.php?title=Part:BBa_K2120201  BBa_K2120201]; [https://parts.igem.org/wiki/index.php?title=Part:BBa_K2120202  BBa_K2120202] ; [https://parts.igem.org/wiki/index.php?title=Part:BBa_K2120203  BBa_K2120203]], here we listed the mutation in -35 region:
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[[File:BIT-CHINA-PARTS-MUTATION-6.png|600px|thumb|center]]
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[[File:BIT-CHINA-PARTS-MUTATION-2.jpg|600px|thumb|center]]
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[[File:BIT-CHINA-PARTS-MUTATION-3.jpg|600px|thumb|center]]
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[[File:BIT-CHINA-PARTS-MUTATION-4.jpg|600px|thumb|center]]
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[[File:BIT-CHINA-PARTS-MUTATION-5.jpg|600px|thumb|center]]
  
 
<!-- Add more about the biology of this part here
 
<!-- Add more about the biology of this part here

Latest revision as of 16:28, 20 October 2016


mutated ptet-2

tetR repressible promoter. The function is similar with pTet BBa_R0040. We mutated the -35 region and selected one with lower strength.It can be used to control the expression of toxin proteins to avoid leaking out.

A series of Ptet promoters

We designed a killer switch controlled by TetR repressor. When the concentration of inhibitors reduces to a threshold, the downstream in-promoter Ptet will start the transcription of killer gene. After measuring the original promoter strength [Part:BBa_R0040], we found that the activity is too high to be well controlled for expressing killer genes. So we mutated the original promoter and got 4 mutants with lower activity.

Design

We analyzed the promoter region and decided to mutated the -35 region through designing random primers. It can at most ensure the change of promoter’s background activity and maintain the promoter’s character since the tightly binding region with repressor is well-conserved while the tightly binding region with RNA polymerase is changed .

Characterization using RFP

The four mutated promoters were characterized using RFP to measure the level of gene expression. Cells were grown in 1.5 mL tube in LB culture medium. The host we used is E.coli TOP10.

Results

Cells showed Red fluorescence under fluorescence microscopy. Quantitative measurement was carried out through enzyme-labeled instrument. It turned out that the highest activity of mutants is about 500, while the common activity is about 200. The original promoter is 9000.

Fig1. Compared with the original promoter, the promoter strength of mutants Ptet-1, Ptet-2, Ptet-3, Ptet-25 is sharply decreased.

We have submitted four mutated promoters [BBa_K2120200; BBa_K2120201; BBa_K2120202 ; BBa_K2120203], here we listed the mutation in -35 region:

BIT-CHINA-PARTS-MUTATION-6.png
BIT-CHINA-PARTS-MUTATION-2.jpg
BIT-CHINA-PARTS-MUTATION-3.jpg
BIT-CHINA-PARTS-MUTATION-4.jpg
BIT-CHINA-PARTS-MUTATION-5.jpg

Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    COMPATIBLE WITH RFC[12]
  • 21
    COMPATIBLE WITH RFC[21]
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    COMPATIBLE WITH RFC[25]
  • 1000
    COMPATIBLE WITH RFC[1000]