Team:SDU-Denmark/protocols

From 2010.igem.org

(Difference between revisions)
(EX1.2)
(Photosensor characterisation)
Line 652: Line 652:
''Microscopy''<br>
''Microscopy''<br>
-
1. 5uL of bacterial culture is placed in the center of a microscopy slide dimensions 7.5cm x 1.5cm and a cover slide is used to cover the culture.<br>
+
1. 5µL of bacterial culture is placed in the center of a microscopy slide dimensions 7.5cm x 1.5cm and a cover slide is used to cover the culture.<br>
2. To eliminate any flow in the system, which can be mistaken for bacterial motility, the cover slide is sealed with ordinary mail polish.<br>
2. To eliminate any flow in the system, which can be mistaken for bacterial motility, the cover slide is sealed with ordinary mail polish.<br>
3. Samples are examined under the microscope.<br><br>
3. Samples are examined under the microscope.<br><br>
Line 661: Line 661:
''Materials:''<br>
''Materials:''<br>
• LB media<br>
• LB media<br>
-
• Motility buffer (20mM potassium phosphate and 0.1mM EDTA dissolved in ddH2O. indsæt ref.)<br>
+
• Motility buffer (20mM potassium phosphate and 0.1mM EDTA dissolved in ddH2O. '''''indsæt ref.''''')<br>
• 1mM retinal<br>
• 1mM retinal<br>
''Protocol:''
''Protocol:''
Line 671: Line 671:
''Microscopy''<br>
''Microscopy''<br>
-
1. 5uL of bacterial culture is placed in the center of a microscopy slide dimensions 7.5cm x 1.5cm and a cover slide is used to cover the culture.<br>
+
1. 5µL of bacterial culture is placed in the center of a microscopy slide dimensions 7.5cm x 1.5cm and a cover slide is used to cover the culture.<br>
2. To eliminate any flow in the system, which can be mistaken for bacterial motility, the cover slide is sealed with ordinary mail polish.<br>
2. To eliminate any flow in the system, which can be mistaken for bacterial motility, the cover slide is sealed with ordinary mail polish.<br>
3. Samples are examined under the microscope.<br><br>
3. Samples are examined under the microscope.<br><br>

Revision as of 11:13, 26 October 2010