Composite

Part:BBa_K3453170

Designed by: Maeva Cherriere   Group: iGEM20_Evry_Paris-Saclay   (2020-10-24)


Grapevine VvTrnL-UAA Toehold Switch 1.1 with sfGFP

This part is an sfGFP (BBa_I746916) expression cassette under the control of the Grapevine Toehold Switch 1.1 (BBa_K2916050) for sequence-based detection of Vitis vinifera.

It is a technical improvement of BBa_K2916068.

Usage and Biology

As depicted in Figure 1, a toehold switch blocks translation initiation because the RBS and the ATG start codon are embedded in the middle of a hairpin structure maintained by base pairs before and after the start codon [1].


T--Evry Paris-Saclay--toehold-switch.png

Figure 1. Toehold switches principle.

The hairpin can be unfolded upon binding of a trigger RNA thereby exposing the RBS and the ATG start codon and thus permitting translation of the reporter protein. For this to happen, two important design precautions have to be taken: (i) the start codon should be in frame with the reporter gene, and (ii) there should be no in-frame stop codon before the reporter gene.

BBa_K2916068 is a composite part formed by BBa_K2916050, BBa_I746916, BBa_B0010 and BBa_B0012 and was specified with an RFC[10] scar between the parts. The RFC[10] scar TACTAG between the BBa_K2916050 (T7 promoter + grapevine switch 1.1) and BBa_I746916 (sfGFP) introduces a stop codon and leads to premature termination of translation (and thus no expected sfGFP production).

Moreover, the role of the trigger RNA is to bind to the toehold switch and thus unfold the hairpin structure thereby exposing the RBS and the ATG start codon and thus permitting translation of the reporter protein. The binding between the trigger and the switch is dictated by RNA-RNA interactions between complementary base pairs.

In BBa_K2916050 (which is the T7 promoter together with grapevine switch 1.1 used to build the composite part BBa_K2916068 as well as this part BBa_K3453170), the trigger binding region is in the same direction as in the grapevine genome and of the trigger sequences derived from (BBa_K3453081 and BBa_K3453083). As a result, this trigger / switch pair does not interact and is not functional. However, the hairpin structure of the grapevine switch 1.1 is predicted to be unfolded by the reverse complements of the two triggers BBa_K3453082 and BBa_K3453084 (Table 1).


Table 1. Grapevine triggers.
Label Part number Transcriptional units’ part numbers Source
Grapevine trigger 'short' BBa_K3453081 BBa_K3453181 EPFL 2019 iGEM team personal communication
Grapevine trigger 'short reverse' BBa_K3453082 BBa_K3453182 Reverse complement of BBa_K3453081
Grapevine trigger 'long' BBa_K3453083 BBa_K3453183 designed by the EPFL 2019 iGEM team and its sequence was deduced from “Amplification” page of the EPFL 2019 wiki where is described how the triggers were designed: the grapevine trigger was PCR amplified using as template the Vitis vinifera TrnL-UAA and the forward primers EC_fwd1 or EC_fwd1_T7 and the EC_rev1 reverse primer (it should be noted that the sequences of all reverse primers listed in the additional materials of this page are given as 3’-5’ sequences and not in the conventional 5’-3’ orientation).
Grapevine trigger 'long reverse' BBa_K3453084 BBa_K3453184 Reverse complement of BBa_K3453083

To circumvent the problems described above, we constructed this part, BBa_K3453170, in which the RFC[10] scar TACTAG was removed by site directed mutagenesis on BBa_K2916068 in pSB3T5 backbone according to Single-Primer Reactions IN Parallel (SPRINP) protocol [2] with the primers 5’-GCTGGCGGCAGCGCAAAAGATGCGTAAAGGCGAAGAGC-3’ and 5’-GCTCTTCGCCTTTACGCATCTTTTGCGCTGCCGCCAGC-3’.

The trigger sequences (Table 1) were placed under the control of the T7 promoter and followed by the strong SBa_000587 synthetic terminator for the T7 RNA polymerase [3] and the resulting transcriptional units were synthesized and assembled in the high copy plasmid pSB1C3.

For toehold switch characterisation we decided to use E. coli BL21 Star™(DE3) cells (Thermo Fisher Scientific), genotype F- ompT hsdSB (rB-mB-) gal dcm rne131 (DE3). As all BL21(DE3) E. coli strains, these cells contain the T7 RNA polymerase under control of the lacUV5 promoter and thus require IPTG to induce expression. The particularity of BL21 Star™(DE3) cells is that they contain a truncated version of the RNaseE gene (rne131) that leads to reduced level of mRNA degradation and thus increased RNA stability. For fluorescence measurements, E. coli cells containing switch and trigger plasmids were first grown overnight in 96-deep-well plates containing 1 mL of LB medium supplemented with 5 µg/mL tetracycline and 17.5 µg/mL chloramphenicol, then diluted by 40x into similar media. Upon reaching early log-phase, cells were further diluted 20x in 100 µL of LB medium supplemented with 5 µg/mL tetracycline, 17.5 µg/mL chloramphenicol and 10 µM IPTG in an opaque wall 96-well polystyrene microplate, the COSTAR 96 (Corning). The plate was incubated at 37°C at 200 rpm and the sfGFP fluorescence (λexcitation 483 nm and λemission 530 nm) and OD600nm were measured every 10 min for 24 hours in a CLARIOstar (BMGLabtech) plate reader. Fluorescence values were normalised by OD600nm and, using the calibration curves presented on the ‘Measurement’ page of our wiki, we converted the arbitrary units into Molecules of Equivalent FLuorescein (MEFL) / particle.

The results presented in figures 2, 3 and 4 show that this part is functional: sfGFP expression was observed only when the BBa_K3453170 was tested in the presence of the two grapevine triggers, both in reverse direction. This confirms that the stop codon introduced by the RFC[10] scar TACTAG plays an important negative role in the function of the toehold switch, as the translation initiated at the AUG codon embedded in the hairpin structure is prematurely stopped before sfGFP translation. Moreover, we can clearly observe that the grapevine switch 1.1 can be activated by a trigger, but only if it is expressed in a reverse complement orientation.

The results presented in Figure 2 show also that the sfGFP expression was readily detected in the positive controls and that the two RBS (BBa_K2675017 and BBa_K3453005) have comparable strength. As expected, no fluorescence was detected in the negative controls as either the sfGFP gene was not present or the promoter and the RBS were absent.



T--Evry Paris-Saclay--MEFL-Particle p26 VvTrnL-UAA1-1.png

Figure 2. In vivo characterization of sfGFP expression by E. coli BL21 Star™(DE3) cells harbouring the grapevine toehold switch 1.1 in BBa_K3453170 and the 'short' and 'long' grapevine triggers in both forward and reverse orientation (BBa_K3453181, BBa_K3453182, BBa_K3453183 and BBa_K3453184). The negative controls have been performed with an empty pSB3T5, pSB1C3 (no trigger) and BBa_K3453103 (no promoter, no RBS) and the positive controls with BBa_K3453104 and BBa_K3453105. The data and error bars are the mean and standard deviation of at least three measurements on independent biological replicates.


T--Evry Paris-Saclay--Fold-change p26 VvTrnL-UAA1-1.png

Figure 3. MEFL / Particle fold changes of the grapevine toehold switch 1.1 in BBa_K3453170 in the presence of the 'short' and 'long' grapevine triggers in both forward and reverse orientation (BBa_K3453181, BBa_K3453182, BBa_K3453183 and BBa_K3453184) compared to the MEFL / Particle value in the absence of the trigger.


T--Evry Paris-Saclay--BoitesFluo p26 VvTrnL-UAA1-1.png

Figure 4: Pictures of E. coli BL21 Star™(DE3) cells harbouring this part and in the presence of the 'short' and 'long' grapevine triggers in both forward and reverse orientation (BBa_K3453181, BBa_K3453182, BBa_K3453183 and BBa_K3453184). The negative control was performed with an empty pSB1C3 (no trigger).


In addition, as the situation turned out to be more complex than expected, we designed two derivatives of the grapevine toehold switch 1.1 denoted 1.1.2 and 1.1.3, three truncated versions laking the trigger binging sites, as well as their cognate sfGFP or sfGFP-LVAtag expression cassettes.

These parts are listed in Table 2 and the results of their characterisation summarised in Figure 5. All details are available on their individual pages in the registry and the full story can be read on the 'Contribution' page of our wiki.


Table 1. Grapevine toehold switches 1.1 and derivatives.
Label Toehold Switch Part Number Toehold Switch + sfGFP Part Number Toehold Switch + sfGFP-LVAtag Part Number
Grapevine VvTrnL-UAA Toehold Switch 1.1 BBa_K2916050 BBa_K2916068 & BBa_K3453170 BBa_K3453171
Truncated Grapevine VvTrnL-UAA Switch 1.1 (no trigger binding site) BBa_K3453072 BBa_K3453172
Grapevine VvTrnL-UAA Toehold Switch 1.1.2 BBa_K3453073 BBa_K3453173 BBa_K3453174
Truncated Grapevine VvTrnL-UAA Switch 1.1.2 (no trigger binding site) BBa_K3453075 BBa_K3453175
Grapevine VvTrnL-UAA Toehold Switch 1.1.3 BBa_K3453076 BBa_K3453176 BBa_K3453177
Truncated Grapevine VvTrnL-UAA Switch 1.1.3 (no trigger binding site) BBa_K3453078 BBa_K3453178


T--Evry Paris-Saclay--MEFL-Particle p22-to-p61.png

Figure 5. In vivo characterization of sfGFP expression by E. coli BL21 Star™(DE3) cells harbouring the grapevine toehold switches 1.1 (Table 2) and the 'short' and 'long' grapevine triggers in both forward and reverse orientation (BBa_K3453181, BBa_K3453182, BBa_K3453183 and BBa_K3453184). The negative controls have been performed with an empty pSB3T5, pSB1C3 (no trigger) and BBa_K3453103 (no promoter, no RBS) and the positive controls with BBa_K3453104 and BBa_K3453105. The data and error bars are the mean and standard deviation of at least three measurements on independent biological replicates.


This BBa_K3453170, as well as BBa_K3453171, BBa_K3453173, BBa_K3453174, BBa_K3453176 and BBa_K3453177 are technical improvements of BBa_K2916068. However, all these six improved parts are functional in the presence of a trigger artificially expressed in E. coli in reverse orientation. They are not able to detect the presence of an RNA naturally expressed in grapevine because the trigger binding site is not in a compatible orientation. But that is another story, and we invite the reader to discover it on the 'Improvement' page of our wiki.

References

[1] Green AA, Silver PA, Collins JJ, Yin P. Toehold switches: de-novo-designed regulators of gene expression. Cell (2014) 159, 925-939.

[2] Edelheit O, Hanukoglu A, Hanukoglu I. Simple and efficient site-directed mutagenesis using two single-primer reactions in parallel to generate mutants for protein structure-function studies. BMC biotechnology (2009) 9, 61.


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
    INCOMPATIBLE WITH RFC[1000]
    Illegal BsaI.rc site found at 53
    Illegal SapI.rc site found at 138


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Categories
Parameters
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