Latest revision as of 16:24, 28 October 2008

Newcastle University

GOLD MEDAL WINNER 2008

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Wet lab work was carried out from 4 August to 19 September, Mondays to Fridays. Please click on a day to see the lab notebook.

Stock pGFPrrnB from -80˚C was plated onto ampicillin, spectinomycin and normal agar (control) and incubated overnight at 37˚C.

2μl pUC57-ncl08 and pJWV021 were run on gel to check quantity. This showed large quantities of both plasmids and therefore pUC57-ncl08 was restricted with EcoRI + NHeI and NHeI + BglII. Controls (buffer A and buffer M without enzyme) were used for both restrictions.

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 ==Friday 22nd August==
-* Stock pGFPrrnB from -80˚C was plated onto ampicillin, spectinomycin and normal [[agar]] (control) and incubated overnight at 37˚C.
+* Stock pGFPrrnB from -80˚C was plated onto ampicillin, spectinomycin and normal [[Making Agar Plates|agar]] (control) and incubated overnight at 37˚C.
-* 2μl pUC57-ncl08 and pJWV021 were run on [[gel]] to check quantity. This showed large quantities of both plasmids and therefore pUC57-ncl08 was [[restricted]] with EcoRI + NHeI and NHeI + BglII. Controls (buffer A and buffer M without enzyme) were used for both restrictions.
+* 2μl pUC57-ncl08 and pJWV021 were run on [[Agarose Gel Electrophoresis|gel]] to check quantity. This showed large quantities of both plasmids and therefore pUC57-ncl08 was [[Restricting Plasmids (Double Restriction)|restricted]] with EcoRI + NHeI and NHeI + BglII. Controls (buffer A and buffer M without enzyme) were used for both restrictions.