Team:SDU-Denmark/protocols

From 2010.igem.org

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Materials
Materials
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•        LB media
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•        LB media <br>
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•        LA plates
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•        LA plates <br>
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•        LA plates with appropriate antibiotic
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•        LA plates with appropriate antibiotic<br>
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•        0.9% NaCl
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•        0.9% NaCl<br>
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2.      The culture is incubated over night at 30°C and 180rpm
2.      The culture is incubated over night at 30°C and 180rpm
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3.      100µL of the culture is serial diluted in 900µL 0.9% NaCl until a dilution of 107 is reached.
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3.      100µL of the culture is serial diluted in 900µL 0.9% NaCl until a dilution of 10<sup>7</sup> is reached.
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4.      100µL of the 105, 106 and 107 dilution is spreaded on LA plates, and LA plates with the appropriate antibiotic, respectively.
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4.      100µL of the 10<sup>5</sup>, 10<sup>6</sup> and 10<sup>7</sup> dilutiona are spread onto LA plates, and LA plates with the appropriate antibiotic, respectively.
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5.      Plates are incubated at 37°C for 16-24 hours. The following day the colonies formed on the plates are counted and cfu are determined.
5.      Plates are incubated at 37°C for 16-24 hours. The following day the colonies formed on the plates are counted and cfu are determined.
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6.      500uL of the 105 dilution is added to 4.5mL of fresh LB media without any antibiotics.
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6.      500µL of the 10<sup>5</sup> dilution is added to 4.5mL of fresh LB media without any antibiotics.
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7.      The new culture is incubated over night at 30°C and 180rpm
7.      The new culture is incubated over night at 30°C and 180rpm
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8.      The experiment is carried out for 5 days. (NB: antibiotic is only added to the first culture. The remaining days the bacteria are grown in cultures without any antibiotics)
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8.      The experiment is carried out for 5 days.  
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(NB: antibiotic is only added to the first culture. The remaining days the bacteria are grown in cultures without any antibiotics)
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Revision as of 18:50, 23 October 2010