Team:Illinois/MicA

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Contents 1 MicA Target-GFP Fusion 2 June 12 3 June 16 4 June 17

MicA Target-GFP Fusion

Purpose: to test the efficiency of sRNA repression. This will be accomplished by forming two plasmids by ligating the target sequence of the sRNA onto the pXG-10 plasmid behind the reporter gene GFP and ligating the sRNA gene into the pJU-334 DNA strand. These plasmids will then be transformed into E. coli and the fluorescence measured with a plate reader.

Protocol(s) Used: The protocol we used is that taken from Urban and Vogel, "A Green Fluorescent Protein (GFP)-Based Plasmid System to Study Post-Transcriptional Control of Gene Expression In Vivo"

Recipe(s) Used:

Primers Used: Forward Primer: GAA AGA CGC GCA TTT GTT ATC

Temp: (4*9) + (2*12) = 60 degrees

Second homology sequence: TTC CAG CCA CAC CGC AAA CGG ((TTCGGTATCA))

Reverse complement: CCG TTT GCG GTG TGG CTG G
Temp: (4*13) + (2*6) = 64 degrees
Cut site and overhang: GTTTTT TCTAGA 

Reverse Primer: GTTTTT TCTAGA CCG TTT GCG GTG TGG CTG G

June 12

Journal entry text goes here.

June 16

We used PCR to extract the sRNA gene: MicA and target sequence : ompA. from the e.coli chromosome. We then ran a gel to make sure that we had the right DNA fragments. Our results corresponded to our predictions.

June 17

We are completing a digestion of MicA, OmpA, and OmpF. Following the digestion we will incubate with SAP and then run a gel to verify the digestion. We will then extract the DNA for the sRNA target sequence and sRNA gene.

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