Team:Heidelberg/Notebook/miRNA Kit/September
From 2010.igem.org
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*inoculation and colony PCR of the transformed (23A+33A)=56C construct from yesterday. Same PCR protocol was used, even though the fragment should be 1100 and therefore elongation was probably not long enough. The PCR showed a band at 300bp, which dominik says is normal if you have religated vector. But nevertheless, miniprep of La1, La3 and La4 were made, because they didn't show a strong negative PCR band. | *inoculation and colony PCR of the transformed (23A+33A)=56C construct from yesterday. Same PCR protocol was used, even though the fragment should be 1100 and therefore elongation was probably not long enough. The PCR showed a band at 300bp, which dominik says is normal if you have religated vector. But nevertheless, miniprep of La1, La3 and La4 were made, because they didn't show a strong negative PCR band. | ||
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* ligation of R56C + R8 + backbone A | * ligation of R56C + R8 + backbone A | ||
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===25/09/2010=== | ===25/09/2010=== | ||
* PCR amplification of standardised pcDNA5 p55 and p1 with primer D47/48 and D55/69 | * PCR amplification of standardised pcDNA5 p55 and p1 with primer D47/48 and D55/69 |
Revision as of 22:12, 25 October 2010
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