Team:Arizona State/Notebook/PCRLog
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<b>CasABCDE</b>: 68 Touchdown from 72 to 65, -.2/cycle, 35 cycles, 2:10 elongation | <b>CasABCDE</b>: 68 Touchdown from 72 to 65, -.2/cycle, 35 cycles, 2:10 elongation | ||
<p>Gel Results:</p> | <p>Gel Results:</p> | ||
- | [[Image:]] | + | [[Image:ASU_729_PCR.jpg|300px]] |
<br>No good | <br>No good | ||
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<b>Cas3</b>: Ran Cas3724 protocol | <b>Cas3</b>: Ran Cas3724 protocol | ||
<p>Gel Results:</p> | <p>Gel Results:</p> | ||
- | [[Image:]] | + | [[Image: ASU_89_CasABCDE.jpg|300px]] |
<br>new: no good | <br>new: no good | ||
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===August 4, 2011=== | ===August 4, 2011=== | ||
<p><b>Settings</b>: 98 initial denaturation for 30 seconds, Cycle (10sec at 98deg, anneal 30 sec at 63 deg, elongate 130sec at 72deg), 35 Cycles, Extension for 450 seconds</p> | <p><b>Settings</b>: 98 initial denaturation for 30 seconds, Cycle (10sec at 98deg, anneal 30 sec at 63 deg, elongate 130sec at 72deg), 35 Cycles, Extension for 450 seconds</p> | ||
- | [[Image:]] | + | [[Image:ASU_PCR_Gel_84.jpg|300px]] |
<br>Results show a band above where we think it ought to be (6 to 8 kbp instead of 4.3) | <br>Results show a band above where we think it ought to be (6 to 8 kbp instead of 4.3) | ||
However, this was extracted and an attempt at a nested PCR was made using the same settings to try and amplify this band even further. The results were blank. | However, this was extracted and an attempt at a nested PCR was made using the same settings to try and amplify this band even further. The results were blank. | ||
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===August 8, 2011=== | ===August 8, 2011=== | ||
<p><b>Settings</b>:ABCDE808, which is same as 8/4 run but only 29 cycles in the hope that the bright band from the previous try would be the only one visible.</p> | <p><b>Settings</b>:ABCDE808, which is same as 8/4 run but only 29 cycles in the hope that the bright band from the previous try would be the only one visible.</p> | ||
- | [[Image:]] | + | [[Image:ASU_88_PCR.jpg|300px]] |
<br>Looks very similar to previous results. Again, a band above where we would like to see it. | <br>Looks very similar to previous results. Again, a band above where we would like to see it. | ||
===August 8, 2011=== | ===August 8, 2011=== | ||
<p><b>Settings</b>: Retry same protocol in thermocycler, however increase back to 35 cycles.</p> | <p><b>Settings</b>: Retry same protocol in thermocycler, however increase back to 35 cycles.</p> | ||
- | [[Image:]] | + | [[Image: ASU_810_Cas3_1.jpg|300px]] |
<br>Not as good as the original run, though there may be faint bands where we would like to see them. For some reason the brightest band is again somewhere between 6k and 8k (though it's a bit hard to tell because the ladder curves annoyingly at the top), instead of the desired 4300. However, we have ordered the nested PCR primers, so perhaps that will offer a better solution to getting Cas ABCDE. In the meantime, we'll focus again on Cas3 and try to extract that and get a good sequencing result so we can say definitively that we have it. | <br>Not as good as the original run, though there may be faint bands where we would like to see them. For some reason the brightest band is again somewhere between 6k and 8k (though it's a bit hard to tell because the ladder curves annoyingly at the top), instead of the desired 4300. However, we have ordered the nested PCR primers, so perhaps that will offer a better solution to getting Cas ABCDE. In the meantime, we'll focus again on Cas3 and try to extract that and get a good sequencing result so we can say definitively that we have it. | ||
===August 10, 2011 (Evening)=== | ===August 10, 2011 (Evening)=== | ||
<p><b>Settings</b>: Ran another PCR for ABCDE, same settings as before but one degree higher for annealing temp. Also added DMSO.</p> | <p><b>Settings</b>: Ran another PCR for ABCDE, same settings as before but one degree higher for annealing temp. Also added DMSO.</p> | ||
- | [[Image:]] | + | [[Image: ASU_810_Cas3_2.jpg|300px]] |
<br>Similar result, less bands from DMSO but consequently much fainter bands. Dimerization still evident. | <br>Similar result, less bands from DMSO but consequently much fainter bands. Dimerization still evident. | ||
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<b>CasABCDE</b>: MgCl2 --> 2uL, 4uL, 5uL, Temp --> 60, 63, 66, 69 | <b>CasABCDE</b>: MgCl2 --> 2uL, 4uL, 5uL, Temp --> 60, 63, 66, 69 | ||
<br><b>Cas3</b>: MgCl2 --> 2uL, 4uL, 5uL, Temp --> 60, 62, 64, 66 | <br><b>Cas3</b>: MgCl2 --> 2uL, 4uL, 5uL, Temp --> 60, 62, 64, 66 | ||
- | [[Image:]] | + | <br>[[Image: ASU_ABCDE_Pranqster.jpeg|300px]] |
<br>CasABCDE: No bands | <br>CasABCDE: No bands | ||
+ | <br>[[Image: ASU_811_Gradient_gel_result.jpeg|300px]] | ||
<br>Cas3: 60 and 62 have bands less than our desired target, up to perhaps 1500; 64 had a couple of bands above this, perhaps one faint one near our 2600 target; 66 had more nonspecific amplification, and no clear bands in our target range | <br>Cas3: 60 and 62 have bands less than our desired target, up to perhaps 1500; 64 had a couple of bands above this, perhaps one faint one near our 2600 target; 66 had more nonspecific amplification, and no clear bands in our target range | ||
<p>Moving forward to nested PCR for ABCDE, we will see how this goes. Cas3 we'll have to keep trying…perhaps it may be worth it to try DMSO, longer elongation time, something. Maybe Taq.</p> | <p>Moving forward to nested PCR for ABCDE, we will see how this goes. Cas3 we'll have to keep trying…perhaps it may be worth it to try DMSO, longer elongation time, something. Maybe Taq.</p> | ||
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===August 12, 2011=== | ===August 12, 2011=== | ||
*PCR using Nest primers for ABCDE | *PCR using Nest primers for ABCDE | ||
- | + | :*Tm1: 74, Tm2: 77 --> Anneal at 72 deg (higher than this is not recommended) | |
- | + | :*Used 2-step Phusion protocol | |
- | + | ::*98 deg for 30 sec | |
- | + | ::*{98deg for 10 sec, 72 deg for 2:30} X 35 cycles | |
- | + | ::*Extension for 7:30 at 72 deg | |
- | + | ::*Held at 4deg until run was cancelled | |
<br>Gel Results: | <br>Gel Results: | ||
- | [[Image:]] | + | <br>[[Image:ASU_812_Nest.jpeg|300px]] |
<br>The 8x MgCl2 tube has the best result | <br>The 8x MgCl2 tube has the best result | ||
<br>Nice clear bands at around 600, 1k, 2k, 4k, 6k, 8k | <br>Nice clear bands at around 600, 1k, 2k, 4k, 6k, 8k | ||
<br>PLAN: use this as template for ABCDE PCR | <br>PLAN: use this as template for ABCDE PCR | ||
<br>Use 1uL per tube (note, we don't know the concentration of the strand we want as template, so this is our best guess as to what would get us between 1pg and 10ng as recommended by the Phusion protocol for non-genomic DNA) | <br>Use 1uL per tube (note, we don't know the concentration of the strand we want as template, so this is our best guess as to what would get us between 1pg and 10ng as recommended by the Phusion protocol for non-genomic DNA) | ||
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Latest revision as of 04:31, 29 September 2011