Team:Austin Texas/kit

From 2014.igem.org

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(Motivation)
(Fidelity of Incorporation)
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''italics = methods Strains containing pFRY and pStG plasmids were grown in the presence and absence of the corresponding non-canonical amino acid. The fluorescence of RFP and GFP readings of each culture were recorded at a culture density of 0.5 OD 600.''  
''italics = methods Strains containing pFRY and pStG plasmids were grown in the presence and absence of the corresponding non-canonical amino acid. The fluorescence of RFP and GFP readings of each culture were recorded at a culture density of 0.5 OD 600.''  
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*This part below is confusing.  I would setup the paragraph... "to deterimine _____, the GFP values of each culture were..."
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GFP values of each culture were normalized to RFP values for analysis. The normalized GFP values were compared between cultures grown in the presence of ncAA and cultures grown in the absence of ncAA. Assuming (+) ncAA cultures showed the higher GFP fluorescence, the greater difference in GFP fluorescence between (+/-) ncAA cultures, the more accurate the ncAA synthetase/tRNA pair.
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To determine the change in GFP fluorescence when the ncAA was present, we first had to calculate how much GFP was expressed relative to the RFP, which would give an upper estimate of how much GFP could theoretically be expressed. We first divided both the GFP and RFP levels by the OD 600 of the culture in order to get the per cell fluorescence levels. We then normalized the GFP fluorescence for one culture to its RFP fluorescence so that we could compare the GFP fluorescence levels between cultures. The normalized GFP values were then compared between cultures grown in the presence of ncAA and cultures grown in the absence of ncAA, which would indicate how the level of GFP fluorescence changes when the ncAA is present. When these values were graphed (Figure 3), some synthetase/tRNA pairs such as 4-azidophenylalanine, 3-nitrotyrosine, 3-iodotyrosine, and ortho-nitrobenzyltyrosine resulted in higher GFP fluorescence in the presence of ncAA than in the absence of ncAA, which suggests that those synthetases only incorporated an amino acid if their specific amino acid was present, meaning that they have a high fidelity. However, the other synthetase/tRNA pairs (3-aminotyrosine, L-DOPA, and cyanophenylalanine) did not show a significant increase in GFP fluorescence normalized to RFP fluorescence when the ncAA was present, indicating that they would incorporate other amino acids at the amber stop codon when their specific amino acid was not present (and perhaps even when it was), and thus have a low fidelity.
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*Then, you can go into this paragraph, and describe what we actually see... which synthetases work well/poorly.  '''You will need to explicitly say what bars you are comparing and how/why you are making your assessment.'''
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Most ncAA synthetase/tRNA pairs resulted in higher GFP fluorescence in the presence of ncAA than in the absence of ncAA, with the exception of 3-aminotyrosine. This suggests that 3-aminotyrosine synthetase/tRNA pair is the least accurate pair from the library tested.
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==Synthetase efficiency==
==Synthetase efficiency==

Revision as of 00:49, 17 October 2014