Team:SDU-Denmark/labnotes2

From 2010.igem.org

(Difference between revisions)
(Purification of pSB1A2 containing J13002)
(Amplification of pSB1A2 w. J13002, pSB1A2 w. B0015 and pSB1A2 w. B0034)
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7: hold 4°C  
7: hold 4°C  
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the experiment for each biobrick was do in duplicats.  
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the experiment for each biobrick was do in duplicats.<br><br>
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''Results:''After amplification the nucleic acid concentration was measured on the Nano Drop. The concentrations was measued to:
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<br><br>
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''Results:''<br><br> After amplification the nucleic acid concentration was measured on the Nano Drop. The concentrations was measued to:
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tube 1: pSB1A2 w. J13002 was 825.2ng/uL
tube 1: pSB1A2 w. J13002 was 825.2ng/uL
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During the DNA extraction 50uL DNA anf 7uL loading buffer was loaded in a lane. The samples was loaded from left to right in continuous numbers.  
During the DNA extraction 50uL DNA anf 7uL loading buffer was loaded in a lane. The samples was loaded from left to right in continuous numbers.  
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The concentration of the extracted DNA from tube 1,2 and  was found to 13.60ng/uL, 16,58ng/uL and 12,6313.60ng/uL respectively. while we have to use the dobbelt terminator and the constitutive active promotor in a lot of experiment the next step is to do another round of PRC and DNA extraction on thise biobricks.  
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The concentration of the extracted DNA from tube 1,2 and  was found to 13.60ng/uL, 16,58ng/uL and 12,6313.60ng/uL respectively. while we have to use the dobbelt terminator and the constitutive active promotor in a lot of experiment the next step is to do another round of PRC and DNA extraction on thise biobricks.<br><br> 
--[[User:Pernm07|Pernm07]] 10:06, 22 July 2010 (UTC)
--[[User:Pernm07|Pernm07]] 10:06, 22 July 2010 (UTC)

Revision as of 10:09, 22 July 2010