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Team:Paris/August 14
From 2008.igem.org
(Difference between revisions)
(→PCR screening of cloning of E0240, flhD, flhC and pflhDC+flhDC) |
(→PCR screening of cloning of E0240, flhD, flhC and pflhDC+flhDC) |
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==PCR screening of cloning of E0240, flhD, flhC and pflhDC+flhDC== | ==PCR screening of cloning of E0240, flhD, flhC and pflhDC+flhDC== | ||
| - | *PCR screening programm | + | *PCR screening programm ; elongation time: 1 min 30 |
| - | + | *total volume reaction: 50 µL | |
| - | *total volume reaction: 50 | + | |
*primers: O18 & O19 | *primers: O18 & O19 | ||
| - | *positive control 1: E0240 | + | *'''positive control 1''': E0240 |
| - | *positive control 2: pSB3K3 | + | *'''positive control 2''': pSB3K3 |
| - | *negative control: no template | + | *'''negative control''': no template |
=> Analysis of the results on [[Team:Paris/August_15|Tomorrow]] | => Analysis of the results on [[Team:Paris/August_15|Tomorrow]] | ||
Revision as of 17:45, 15 August 2008
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Results of the PCR of the wonderful promoter of fliL
Remarks: We observe that the bands are curved, we suppose that the wells were not very clean. The size of fliL is good, we will digest it and ligate it today. Digestion and Ligation of the wonderful promoter of fliLAs the primer used to amplify the promoter of fliL had only two nucleotides after the restriction sites, we tried the two digestions possible : EcoRI + SpeI and XbaI + PstI. DigestionProtocol :
Washing of the digestionsWe washed the DNA following the standard protocol. Ligation
PCR screening of cloning of E0240, flhD, flhC and pflhDC+flhDC
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