Part:BBa_K567012
tRNA(Asp)-AGG
tRNAArg with its anticodon mutated to CCU(base pairing rare codon AGG) and under the control of aspV promoter. This biobrick is constructed first by cloning the tRNAArg from aspV in E.coli, then the anticodon region is site-directed mutated.
This part is worked coordinately with TDRS(BBa_K567011). TDRS is aspartyl aminoacyl tRNA synthetase without anticodon recognition domain. This modified AspRS can charge Asp to tRNAAsp-AGG (BBa_K567012). With tRNAAsp-AGG and TDRS, the ribosome can get through consecutive AGG codons on the mRNA.
Reporter:We test our design with two reporters.
RFP-6AGG (BBa_K567017) : RFP with 6AGG insertions
Luciferase-4AGG (BBa_K567009) : luciferase with 4AGG insertions
When the modified enzyme is produced under induction, it can charge tRNAAsp-AGG with Arg. Then the charged tRNA can get through the rare codons on the mRNA, so that RFP or luciferase can be produced.
We have used PT7-RFP-6AGG (BBa_K567017) as our Reporter. We have constructed tRNAAsp-AGG and PT7-TDRS (AspRS without anticodon recognition domain) (BBa_K567012 and BBa_K567011). tRNAAsp-AGG, which can recognize rare codon AGG, is under constitutive promoter. With our device, RFP is successfully produced. Without our device, little RFP is observed.
We have used PT7-Luc-4AGG (BBa_K567009) as our Reporter to test the function of PT7-TDRS (BBa_K567011) and tRNAAsp-AGG (BBa_K567012). Results are shown above. Luciferase production has been largely increased with our device.
Get more information from Biobrick
PT7-TDRS (BBa_K567011)
Sequence and Features
- 10INCOMPATIBLE WITH RFC[10]Illegal EcoRI site found at 281
- 12INCOMPATIBLE WITH RFC[12]Illegal EcoRI site found at 281
- 21INCOMPATIBLE WITH RFC[21]Illegal EcoRI site found at 281
- 23INCOMPATIBLE WITH RFC[23]Illegal EcoRI site found at 281
- 25INCOMPATIBLE WITH RFC[25]Illegal EcoRI site found at 281
- 1000COMPATIBLE WITH RFC[1000]
| chassis | Escherichia coli |