SBB11Ntbk-Averee Chang: Difference between revisions
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My PCR product came back today (the one I re-did yesterday to make parts P-narP and P-sfmC) and I am currently running an analytical gel to ensure that my part got successfully amplified. To prepare for the analytical gel, I added 2.5 μL of blue dye and 6μL of the part for each part. <br> | My PCR product came back today (the one I re-did yesterday to make parts P-narP and P-sfmC) and I am currently running an analytical gel to ensure that my part got successfully amplified. To prepare for the analytical gel, I added 2.5 μL of blue dye and 6μL of the part for each part. <br> | ||
When the gel picture came back, [http://openwetware.org/wiki/Image:021811-AnalGel1.jpg | When the gel picture came back, [http://openwetware.org/wiki/Image:021811-AnalGel1.jpg Analytical Gel 1], my PCRs seemed successful. My two columns, column 9 and column 10 which are the last two on the far right, have bands at around 650 and 850 bp. This correlates with my part's length, 620bp for P_sfmC and 723bp for P-narP <br> | ||
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Revision as of 14:38, 18 February 2011
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Averee Chang 15:56, 18 February 2011 (EST)
I gel purified the part I digested with EcoRI and BamHI, jtk2914, using the protocol Zymo Gel Purification.
My PCR product came back today (the one I re-did yesterday to make parts P-narP and P-sfmC) and I am currently running an analytical gel to ensure that my part got successfully amplified. To prepare for the analytical gel, I added 2.5 μL of blue dye and 6μL of the part for each part.
When the gel picture came back, Analytical Gel 1, my PCRs seemed successful. My two columns, column 9 and column 10 which are the last two on the far right, have bands at around 650 and 850 bp. This correlates with my part's length, 620bp for P_sfmC and 723bp for P-narP
Averee Chang 13:03, 3 February 2011 (EST)
Tuesday (February 15): Did a PCR to make P_narP from oligos ss34F, ss34R and P_sfmC from oligos ss52F,ss52R. Today, my PCR yield had too little volume (probably due to a loose cap on the PCR tube) and I re-did the PCR for both of them today using protocol Cloning by PCR
Today, along with re-doing the two PCRs, I digested part jtk2914 from pBjh1601KC-jtk2914 using EcoRI and BamHI. After doing a preparation gel, I cut out the larger band of the two and melted the agarose gel and froze it in box "C." I digested with EcoRI/BamHI and underwent the preparation gel using EcoRI/BamHI Digest of PCR Products
