Team:UChicago/Plan

From 2013.igem.org

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== '''Construct pUB110 BioBrick''' ==
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pUB110 BioBrick
 
-Digest pUB110 w/ NdeI and AflII--> gel purify-->nanodrop for concentration
-Digest pUB110 w/ NdeI and AflII--> gel purify-->nanodrop for concentration
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 +
-Digest pUB110 linker w/ NdeI and AflII
-Digest pUB110 linker w/ NdeI and AflII
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linker:  
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 +
 
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Linker sequence:  
attcgtcttaaggaattcgcggccgcttctagagtactagtagcggccgctgcagcatatgtcatac
attcgtcttaaggaattcgcggccgcttctagagtactagtagcggccgctgcagcatatgtcatac
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gtatgacatatgctgcagcggccgctactagtactctagaagcggccgcgaattccttaagacgaat
 
-Set up overnight ligation of digested, gel purified pUB110 and digested pUB110 linker = generates pUB110 BioBrick
-Set up overnight ligation of digested, gel purified pUB110 and digested pUB110 linker = generates pUB110 BioBrick
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-Transform into B. subtilis to amplify
-Transform into B. subtilis to amplify
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-Set up O. N. cultures
-Set up O. N. cultures
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-Do B. subtilis miniprep
-Do B. subtilis miniprep
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-Digest our pUB110 BioBrick  
-Digest our pUB110 BioBrick  
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To test pUB110 Biobrick (kanamycin resistant) construction (send for sequencing)
To test pUB110 Biobrick (kanamycin resistant) construction (send for sequencing)
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-Put a promoter/upstream BioBrick (in vector with chloramphenicol resistance) + RFP BioBrick from amp resistant vector => do 3 step assembly  
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-Put a promoter/upstream BioBrick (in vector with chloramphenicol resistance) + RFP BioBrick from amp resistant vector => do 3 step assembly
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 +
-Do transformation in B. subtilis
-Do transformation in B. subtilis
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-Choose transformants--> if transformants express RFP, we could conclude our pUB110 BioBrick works--> submit pUB110 BioBrick
-Choose transformants--> if transformants express RFP, we could conclude our pUB110 BioBrick works--> submit pUB110 BioBrick
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kerA BioBrick
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== "Construct kerA BioBrick" ==
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-Do Gibson assembly to put together the two kerA gBlocks from IDT
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-Put our kerA biobrick into an empty vector w/ amp resistance (so we can use the 3 step assembly) and transform into DH5-a
-Put our kerA biobrick into an empty vector w/ amp resistance (so we can use the 3 step assembly) and transform into DH5-a
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 +
-Since promoter/upstream biobrick will be in chloramphenicol resistant vector
-Since promoter/upstream biobrick will be in chloramphenicol resistant vector
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 +
-And our puB110 vector will use kanamycin resistance
-And our puB110 vector will use kanamycin resistance
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 +
-So that leaves our kerA biobrick the vector that is amp resistant
-So that leaves our kerA biobrick the vector that is amp resistant
Orange: prefix
Orange: prefix
Green: suffix
Green: suffix
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Purple: kerA Sac signal peptide
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Purple: kerA signal peptide
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     </div>

Revision as of 19:57, 27 September 2013




== '''Construct pUB110 BioBrick''' == -Digest pUB110 w/ NdeI and AflII--> gel purify-->nanodrop for concentration -Digest pUB110 linker w/ NdeI and AflII Linker sequence: attcgtcttaaggaattcgcggccgcttctagagtactagtagcggccgctgcagcatatgtcatac -Set up overnight ligation of digested, gel purified pUB110 and digested pUB110 linker = generates pUB110 BioBrick -Transform into B. subtilis to amplify -Set up O. N. cultures -Do B. subtilis miniprep -Digest our pUB110 BioBrick To test pUB110 Biobrick (kanamycin resistant) construction (send for sequencing) -Put a promoter/upstream BioBrick (in vector with chloramphenicol resistance) + RFP BioBrick from amp resistant vector => do 3 step assembly -Do transformation in B. subtilis -Choose transformants--> if transformants express RFP, we could conclude our pUB110 BioBrick works--> submit pUB110 BioBrick == "Construct kerA BioBrick" == -Do Gibson assembly to put together the two kerA gBlocks from IDT -Put our kerA biobrick into an empty vector w/ amp resistance (so we can use the 3 step assembly) and transform into DH5-a -Since promoter/upstream biobrick will be in chloramphenicol resistant vector -And our puB110 vector will use kanamycin resistance -So that leaves our kerA biobrick the vector that is amp resistant Orange: prefix Green: suffix Purple: kerA signal peptide