BBa_K2009602

BBa_K2009602 Version 1

Component

Source:
http://parts.igem.org/Part:BBa_K2009602
Generated By: https://synbiohub.org/public/igem/igem2sbol/1
Created by: Yin Wu
Date created: 2016-09-13 11:00:00
Date modified: 2016-09-17 07:37:40

sfGFP11 with promoter and RBS



    • Details

    Types
    DnaRegion

    Roles
    Composite

    engineered_region

    Sequences BBa_K2009602_sequence (Version 1)

    Description

    sfGFP11 length: 112bp
    Derived from:synthesis from Sangon
    BBa_J23100: promoter:

    BBa_B0030: RBS

    sfGFP11??????PSB1C3 is an expression plasmid which insert sfGFP11 into PSB1C3.

    before sfGFP11, we add a linker(gatggagggtctggtggcggatca) to achieve our goal.SfGFP11 is a part of GFP(from 214bp to 230bp), GFP has been mutated to improve its solubilityand self-associating activity. When it express, it will emit green fluorescenceslightly under the fluorescence microscope.

    We try to find anideal protein tag to be work both invivo and invitro and it can provide a sensitive measurable signalwhich don???t need external chemical reagents or substrates. Finally we find away to accomplish this goal?????? dividing GFP into sfGFP1-10and sfGFP11. Either the sfGFP1-10 or sfGFP11 will emit green fluorescence slightly under the fluorescencemicroscope. However, when sfGFP1-10 and sfGFP11 express insame cell, they will interact each other and emit more intense fluorescence thaneach of them. The split GFP system is simple and does not change fusion proteinsolubility.

    Usage and biology:The split GFP system has manypractical applications. Obtaining soluble, well-folded recombinant proteins fordownstream applications requires screening large numbers of protein variants (mutants,fragments, fusion tags, folding partners) and testing many expression orrefolding conditions.(Ste??phanieCabantous, Thomas C Terwilliger & Geoffrey S Waldo,2005)

    Part sequence

    ttgacggctagctcagtcctaggtacagtgctagctactagagattaaagaggagaaatactagagagaccacatggtccttcatgagtatgtaaatgctgctgggattaca
    (All the sequence has been testified by Sangon)

    Notes

    If we PCR from GFP directly, we have to mutate it many times and it is more convenient to directly synthese it.

    Source

    chenical synthesis and link it to BBa_K081005

    Access Instance Definition
    public
    public
    		BBa_K081005
    BBa_K2009820
    		BBa_K081005
    sfGFP11

    Sequence Annotation Location Component / Role(s)
    BBa_K081005
    BBa_K2009820
    		1,58
    67,114
    		BBa_K081005
    sfGFP11

    igem#experience
    None
     
    igem#status
    Planning
     
    synbiohub#ownedBy
    user/james
     
    synbiohub#ownedBy
    user/myers
     
    synbiohub#topLevel
    BBa_K2009602/1
     

    Attachments

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