Team:Austin Texas/kit

From 2014.igem.org

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(Experimental Design and Method)
(Experimental Design and Method)
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A total of seven ncAAs were used in addition to tyrosine.  [https://2014.igem.org/Team:Austin_Texas/kit#ncAA_Table The full list of amino acids used in this study can be found here].
A total of seven ncAAs were used in addition to tyrosine.  [https://2014.igem.org/Team:Austin_Texas/kit#ncAA_Table The full list of amino acids used in this study can be found here].
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The kit consists of a three plasmid system: pBLG, pFRYC, and pFRY. pBLG contains the ncAA synthetase/tRNA pair to be tested as well as a gentamicin resistance gene. pFRYC is the control plasmid and contains the IPTG-induced reporter system and a kanamycin resistance gene. The reporter system is composed of RFP and sfGFP fused via a linker sequence between the two. pFRY is the experimental plasmid and is nearly identical to pFRYC with the exception that its linker sequence contains an amber stop codon in the middle of the linker whereas pFRYC contains a codon for tyrosine in the same location. In a cell containing pFRYC, the ribosome will translate the RFP reporter, linker, and finally sfGFP, producing red and green fluorescent proteins that result in visible yellow fluorescence. In a cell containing pFRY, the ribosome will translate the sfGFP and terminate at the amber stop codon on the linker producing a green fluorescence. When pBLG and pFRY are present in the cell, the ribosome will incorporate an ncAA at the amber codon in the linker and continue translation producing both RFP and sfGFP reporters if the synthetase/tRNA pair encoded on pBLG effectively incorporate the ncAA.
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[[File:Kit Plasmid Alignment 10-14-14.png|600px|thumb|center|Figure 2. pStG contains the specific ncAA synthetase/tRNA pair being tested. pFRYC and pFRY are the ncAA kit reporter plasmids.  pFRYC is the control plasmid that yields GFP and RFP expression regardless of synthetase/tRNA pair. pFRY is a nearly identical plasmid with a single difference, the linker between the GFP and RFP sequences contains an amber codon in place of the tyrosine codon found in pFRYC. Thus, the level of GFP expression for pFRY is directly dependent on the efficiency and fidelity of the synthetase/tRNA pair being tested.]]
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D)      (+) ncAA Synthetase/tRNA pair, (+) ncAA.]]
D)      (+) ncAA Synthetase/tRNA pair, (+) ncAA.]]
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The kit consists of a three plasmid system: pBLG, pFRYC, and pFRY. pBLG contains the ncAA synthetase/tRNA pair to be tested as well as a gentamicin resistance gene. pFRYC is the control plasmid and contains the IPTG-induced reporter system and a kanamycin resistance gene. The reporter system is composed of RFP and sfGFP fused via a linker sequence between the two. pFRY is the experimental plasmid and is nearly identical to pFRYC with the exception that its linker sequence contains an amber stop codon in the middle of the linker whereas pFRYC contains a codon for tyrosine in the same location. In a cell containing pFRYC, the ribosome will translate the RFP reporter, linker, and finally sfGFP, producing red and green fluorescent proteins that result in visible yellow fluorescence. In a cell containing pFRY, the ribosome will translate the sfGFP and terminate at the amber stop codon on the linker producing a green fluorescence. When pBLG and pFRY are present in the cell, the ribosome will incorporate an ncAA at the amber codon in the linker and continue translation producing both RFP and sfGFP reporters if the synthetase/tRNA pair encoded on pBLG effectively incorporate the ncAA.
 
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[[File:Kit Plasmid Alignment 10-14-14.png|600px|thumb|right|Figure 2.  Plasmids used in the ncAA kit.'''KATE, FIX the "pBIG" to BLG  ALSO NO STOP CODON???-Dennis''' ''Also, I would rotate the FRY plasmids 90º and BLG so the synthetase and tRNA sit top-middle and gent on the bottom-middle, remove the arrowhead on lacO and make it as narrow as the text, it's an operator, not a gene, and consider changing the name of BLG, the L was for lacI and that was moved to the FRY plasmids, right?-Jordan'' pBLG contains the specific synthetase/tRNA pair being tested. pFRYC and pFRY are the ncAA kit reporter plasmids.  pFRYC is the control plasmid that yields GFP and RFP expression regardless of synthetase/tRNA pair. pFRY is a nearly identical plasmid with a single difference, the linker between the GFP and RFP sequences contains an amber codon in place of the tyrosine codon found in pFRYC. Thus, the level of GFP expression for pFRY is directly dependent on the efficiency and fidelity of the synthetase/tRNA pair being tested.]]
 

Revision as of 17:24, 14 October 2014