Team:ESBS-Strasbourg/Concentrations Measurements

From 2008.igem.org

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'''1)by spectrophotometer'''
'''1)by spectrophotometer'''
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step1: Prepare your sample:
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step1: Prepare your sample: <br>
2µL of the solution <br>
2µL of the solution <br>
400µL Water <br>
400µL Water <br>
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step2: put lambda=260nm <br>
step2: put lambda=260nm <br>
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step3: do the blank with the same water you used for dilution <br>
step3: do the blank with the same water you used for dilution <br>
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step4: Do the conversion absorbance->concentrations <br>
step4: Do the conversion absorbance->concentrations <br>
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=>Multiply your DO per 50, and then per 200 for the dilution factor. Then you have your DNA concentrations in ng/µL. <br>
=>Multiply your DO per 50, and then per 200 for the dilution factor. Then you have your DNA concentrations in ng/µL. <br>
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'''By nanodrop'''
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'''2)By nanodrop'''
Ask Maria to use it at the Pharma faculty. You only need 1µL of your solution. <br>
Ask Maria to use it at the Pharma faculty. You only need 1µL of your solution. <br>
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[[Team:ESBS-Strasbourg/Protocols|''Protocols'']]

Latest revision as of 13:09, 29 July 2008

1)by spectrophotometer

step1: Prepare your sample:
2µL of the solution
400µL Water


step2: put lambda=260nm


step3: do the blank with the same water you used for dilution


step4: Do the conversion absorbance->concentrations

1DO = 50µgDNA/mL = 50ng/µL

=>Multiply your DO per 50, and then per 200 for the dilution factor. Then you have your DNA concentrations in ng/µL.


2)By nanodrop

Ask Maria to use it at the Pharma faculty. You only need 1µL of your solution.



Protocols