Difference between revisions of "Part:BBa K1379001"

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<partinfo>BBa_K1379001 short</partinfo>
 
<partinfo>BBa_K1379001 short</partinfo>
  
SigmaX-dependent promoter initiating the transcription of helicase in ''Streptococcus pneumoniae'' NCTC7465 strain.
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SigmaX dependent promoter initiating the transcription of helicase in ''Streptococcus pneumoniae'' NCTC7465 strain.  
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Phelicase is a promoter which proves to be functional in E. coli and S. pneumonia. The sigmaX protein will bind to 8 base pairs of Phelicase promoter and trigger gene expression. The sigmaX gene and Phelicase promoter used in the construct are both cloned from E. coli NCTC 7465 strain. R.P.U (Relative Promoter Unit) of Phelicase is measured to represent promoter strength in reference to constitutive promoter [[Part:BBa_J23100|BBa_J23100]]. Phelicase promoter is characterized in E. coli DH10B cell as it is frequently used by iGEM participants.
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<br><br>
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'''<font size="4">Objective</font>'''<br>
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The objective is to characterize Phelicase promoter so we know whether it iss working in ''E. coli'' DH10B strain or not, and to know the R.P.U (Relative Promoter Unit) with [[Part:BBa_J23100|BBa_J23100]] constitutive promoter as a reference.
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<br><br>
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'''<font size="4">Method</font>''' <br>
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By linking Phelicase promoter with GFP generator ([[Part:BBa_E0240|BBa_E0240]]), and SigmaX Generator ([[Part:BBa_K1379006|BBa_K1379006]]), the promoter activity was represented by the GFP synthesis rate. Fluorescence was measured when the cells are in the mid-log phase. OD595 values were measured and converted to OD600 to obtain the R.P.U of the promoter.
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<br><br>
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'''<font size="4">Characterization</font>'''<br>
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To measure the RPU (Relative Promoter Unit) of Phelicase promoter, we adopted the method described by Kelly et al. in “Measuring the activity of BioBrick promoters using an in vivo reference standard” (Kelly et al., 2009). With the use of EnVision multilabel reader from Perkin Elmer Company, it enabled us to obtain the fluorescence and absorbance of cells over time. GFP intensity and OD595 values were measured every 30 minutes after the E. coli strains are cultured to mid-log phase.
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<br><br>
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The positive control used in this characterization is [[Part:BBa_I20260|BBa_I20260]] which is a constitutive promoter [[Part:BBa_J23100|BBa_J23100]] containing GFP generator [[Part:BBa_E0240|BBa_E0240]], while the negative control used in this characterization is [[Part:BBa_K1379003|BBa_K1379003]] which is Phelicase promoter with GFP generator but without SigmaX generator.
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<br><br>
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The detailed description including characterization procedure and Data processing of our characterization can be found in [http://2014.igem.org/Team:Hong_Kong_HKUST/pneumosensor/characterization iGEM HKUST 2014 Wiki Page].
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<br>
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[[File:phelicasepicture.png|500px|thumb|center|'''Figure 1. Phelicase promoter induced by SigmaX protein drives GFP expression. While the same construct without SigmaX protein did not give any GFP signals. Another negative control which is only protein sigmaX without Phelicase also did not give any GFP signals. Reference promoter [[Part:BBa_J23100|BBa_J23100]] + GFP is used as positive control. Scale bar = 5mm.]]
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<br><br>
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[[File:phelicasegraphs.png|700px|thumb|center|'''Figure 2. Phelicase promoter Relative Promoter Unit (RPU) is measured with reference to [[Part:BBa_J23100|BBa_J23100]] constitutive promoter. Phelicase promoter induced by SigmaX protein gave GFP signals. This fluorescence expression was measured over time, and divided by the OD of the cells. In the end, it was standardized based on [[Part:BBa_J23100|BBa_J23100]] promoter strength. Measurement was done by using 3 replicas.]]
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<br><br>
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'''
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==Reference ==
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'''
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J. R. Kelly, A. J. Rubin, J. H. Davis, J. Cumbers, M. J. Czar, ..., D. Endy. (2009). Measuring the activity of BioBrick promoters using an in vivo reference standard. Journal of Biological Engineering, 3, 4. doi: 10.1186/1754-1611-3-4<br><br><br>
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Revision as of 14:59, 7 October 2014

PcomFA

SigmaX dependent promoter initiating the transcription of helicase in Streptococcus pneumoniae NCTC7465 strain. Phelicase is a promoter which proves to be functional in E. coli and S. pneumonia. The sigmaX protein will bind to 8 base pairs of Phelicase promoter and trigger gene expression. The sigmaX gene and Phelicase promoter used in the construct are both cloned from E. coli NCTC 7465 strain. R.P.U (Relative Promoter Unit) of Phelicase is measured to represent promoter strength in reference to constitutive promoter BBa_J23100. Phelicase promoter is characterized in E. coli DH10B cell as it is frequently used by iGEM participants.

Objective

The objective is to characterize Phelicase promoter so we know whether it iss working in E. coli DH10B strain or not, and to know the R.P.U (Relative Promoter Unit) with BBa_J23100 constitutive promoter as a reference.

Method

By linking Phelicase promoter with GFP generator (BBa_E0240), and SigmaX Generator (BBa_K1379006), the promoter activity was represented by the GFP synthesis rate. Fluorescence was measured when the cells are in the mid-log phase. OD595 values were measured and converted to OD600 to obtain the R.P.U of the promoter.

Characterization

To measure the RPU (Relative Promoter Unit) of Phelicase promoter, we adopted the method described by Kelly et al. in “Measuring the activity of BioBrick promoters using an in vivo reference standard” (Kelly et al., 2009). With the use of EnVision multilabel reader from Perkin Elmer Company, it enabled us to obtain the fluorescence and absorbance of cells over time. GFP intensity and OD595 values were measured every 30 minutes after the E. coli strains are cultured to mid-log phase.

The positive control used in this characterization is BBa_I20260 which is a constitutive promoter BBa_J23100 containing GFP generator BBa_E0240, while the negative control used in this characterization is BBa_K1379003 which is Phelicase promoter with GFP generator but without SigmaX generator.

The detailed description including characterization procedure and Data processing of our characterization can be found in [http://2014.igem.org/Team:Hong_Kong_HKUST/pneumosensor/characterization iGEM HKUST 2014 Wiki Page].


Figure 1. Phelicase promoter induced by SigmaX protein drives GFP expression. While the same construct without SigmaX protein did not give any GFP signals. Another negative control which is only protein sigmaX without Phelicase also did not give any GFP signals. Reference promoter BBa_J23100 + GFP is used as positive control. Scale bar = 5mm.



Figure 2. Phelicase promoter Relative Promoter Unit (RPU) is measured with reference to BBa_J23100 constitutive promoter. Phelicase promoter induced by SigmaX protein gave GFP signals. This fluorescence expression was measured over time, and divided by the OD of the cells. In the end, it was standardized based on BBa_J23100 promoter strength. Measurement was done by using 3 replicas.



Reference

J. R. Kelly, A. J. Rubin, J. H. Davis, J. Cumbers, M. J. Czar, ..., D. Endy. (2009). Measuring the activity of BioBrick promoters using an in vivo reference standard. Journal of Biological Engineering, 3, 4. doi: 10.1186/1754-1611-3-4




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]