Edinburgh/13 July 2008


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Sunday 13 July 08

 * Signs of growth on Cellulomonas plates 28 and 29.
 * Minipreps M25 to M30 of possible rbs+dxs clones from plate 34.
 * PCR P12 to obtain rbs+dxs fusion product in case minipreps didn't work. Template was ligation L11, and primers were rbs2clonf1 and pSB1A2insr1. Annealing was 58°C, extension 40s using KOD.
 * M25 to M30 were digested with SacI/SpeI and run on gel 12 along with undigested P12. This shows that M25 to M30 are no good.


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