Team:SDU-Denmark/protocols

From 2010.igem.org

(Difference between revisions)
(PS1.1)
(PS1.1)
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• Diluted LB media<br>
• Diluted LB media<br>
• Difco Agar<br>
• Difco Agar<br>
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1mM retinal<br><br>
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1µM retinal (final concentration)<br><br>
''Swimming motility plates''<br>
''Swimming motility plates''<br>
1. LB media is mixed with 0.3% difco agar and autoclavated<br>
1. LB media is mixed with 0.3% difco agar and autoclavated<br>
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2. The appropriate antibiotic and 1uM retinal is added to the autoclaved media (NB: for the media used for the control plates, no antibiotic or retinal is added)<br>
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2. The appropriate antibiotic and 1µM retinal (final concentration) is added to the autoclaved media (NB: for the media used for the control plates, no antibiotic or retinal is added)<br>
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3. Plates are cast and incubated ON at room temperature<br>
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3. Plates are cast and incubated overnight at room temperature<br>
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4. 15 minutes prior to the experiment the plates are incubated at 37°C.<br><br>
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4. 15 minutes prior to the experiment the plates are dried at 37°C.<br><br>
''Sample preparation''<br>
''Sample preparation''<br>
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1. Colony is inoculated in 5mL LB media containing the appropriate antibiotic. The culture is grown ON at 37°C and 180rpm.<br>
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1. 5mL LB media containing the appropriate antibiotic is inoculated with a colony. The culture is grown overnight at 37°C and 180rpm.<br>
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2. ON culture is diluted in 5mL LB media containing the appropriate antibiotic to reach an OD550 of 0.02 and are incubated at 37°C and 180rpm until it reaches an OD550 of 0.5.<br>  
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2. The overnight culture is diluted in 5mL LB media containing the appropriate antibiotic to reach an OD550 of 0.02 and are incubated at 37°C and 180rpm until it reaches an OD550 of 0.5.<br>  
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3. 1mM retinal is added to the culture (NB: no retinal is added to the cultures containing the control cells)<br>
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3. 1µM retinal (final cnocentration) is added to the culture (NB: no retinal is added to the cultures containing the control cells)<br>
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4. The tubes containing the cultures are wrapped in tin foil and are subsequently grown for 2 hours at 37°C and 180rpm.<br><br>
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4. The tubes containing the cultures are wrapped in tin foil (creates darkness) and are subsequently grown for 2 hours at 37°C and 180rpm.<br><br>
''Motility assay''<br>  
''Motility assay''<br>  
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1. 2x2.5uL of culture is placed on each plate, and the plates are placed in a specially engineered lightbox, so that ½ of each plate is illuminated with blue light and the other ½ is kept in dark. 1mL of each culture is used for microscopy.<br>
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1. 2x2.5µL of culture is placed on each plate, and the plates are placed in a specially engineered lightbox, so that ½ of each plate is illuminated with blue light and the other ½ is kept in dark. <br>
2. The plates are incubated at 37°C for 24 hours.<br>
2. The plates are incubated at 37°C for 24 hours.<br>
3. Pictures are taken<br><br>
3. Pictures are taken<br><br>
''Microscopy''<br>
''Microscopy''<br>
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1. 5uL cell culture is used for the microscopy<br>
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1. 5µL cell culture is used for the microscopy<br>
2. To avoid laminar flow, the microscopy slide is sealed with nail polish.<br>
2. To avoid laminar flow, the microscopy slide is sealed with nail polish.<br>
3. Samples are examined under the microscope.<br><br>
3. Samples are examined under the microscope.<br><br>

Revision as of 17:23, 23 October 2010