BBa_J100219

BBa_J100219 Version 1

Component

Source:
http://parts.igem.org/Part:BBa_J100219
Generated By: https://synbiohub.org/public/igem/igem2sbol/1
Created by: Julia Preziosi
Date created: 2015-06-23 11:00:00
Date modified: 2015-08-31 04:08:24

tCloneTet with Riboswitch 8



    • Details

    Types
    DnaRegion

    Roles
    Device

    engineered_region

    Sequences BBa_J100219_sequence (Version 1)

    Description

    Using Golden Gate Assembly, the transcriptional riboswitch RS8 (from Wachsmuth, et al.) was ligated into the destination vector tClone Tet (J119374) in place of the insert (between BsaI sites). This riboswitch is controlled by theophylline, allowing transcription if theophylline is present. However, it also has shown increased transcription levels in the presence of caffeine. Based on the previous research of Wachsmuth, et al., we do not expect this to be a very effective riboswitch (small dynamic range). We will be using it as a negative control.

    Notes

    The plasmid that this part is located in is pUC-BR, a plasmid modified from pUC-IDT-Amp with an errant BsaI site in the Ampicillin resistance gene removed.

    Source

    Part BBa_J119374, and Wachsmuth et al. 2013, available from http://www.ncbi.nlm.nih.gov/pmc/articles/PMC3575828/ .

    Sequence Annotation Location Component / Role(s)
    P5 promoter
    Riboswitch 8
    BD18 C dog RBS
    TetA
    		1,36
    41,112
    117,201
    202,1398
    		feature/promoter promoter
    feature/stem_loop stem_loop
    feature/rbs ribosome_entry_site
    CDS feature/cds

    igem#sampleStatus
    Not in stock
    igem#status
    Unavailable
     
    synbiohub#ownedBy
    user/james
     
    synbiohub#ownedBy
    user/myers
     
    synbiohub#topLevel
    BBa_J100219/1
     

    Attachments

    © 2018 Newcastle University, University of Utah, and collaborators
    About SynBioHub | View Source on Github | Report an Issue
    | v1.6.1 (86615526)