Difference between revisions of "Team:Marburg/Experiments"

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<h2 class="subtitle">Cultivation</h2>
 
<h2 class="subtitle">Cultivation</h2>
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<li>Measure OD<sub>730nm</sub> to use cells when the OD is between 0.5 and 1.0</li>
 
<li>Measure OD<sub>730nm</sub> to use cells when the OD is between 0.5 and 1.0</li>
 
<li>Spin down cells in sterile tube at 6000 × g at room temperature.</li>
 
<li>Spin down cells in sterile tube at 6000 × g at room temperature.</li>
<li>Concentrate the cells by re-suspending them in smaller amount of fresh growth medium so to
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<li>Concentrate the cells by re-suspending them in smaller amount of fresh growth medium so
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to
 
get
 
get
 
a final OD<sub>730nm</sub> of 2.5 – 3.5</li>
 
a final OD<sub>730nm</sub> of 2.5 – 3.5</li>
 
<li>Place 0.4 mL of re-suspended cells in sterile culture tubes.</li>
 
<li>Place 0.4 mL of re-suspended cells in sterile culture tubes.</li>
<li>Add 50 ng – 2 µg plasmid DNA to each tube and gently mix. (Leave one tube as a control w/o
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<li>Add 50 ng – 2 µg plasmid DNA to each tube and gently mix. (Leave one tube as a control
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w/o
 
DNA
 
DNA
 
added).</li>
 
added).</li>
 
<li>Wrap tubes in aluminum foil (perhaps make hole in Eppie lid for gas exchange).</li>
 
<li>Wrap tubes in aluminum foil (perhaps make hole in Eppie lid for gas exchange).</li>
<li>Place the tubes in the growth chamber at 30° (if high CO2 requiring phenotype is expected
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<li>Place the tubes in the growth chamber at 30° (if high CO2 requiring phenotype is
 +
expected
 
place plates in 3 % CO2) for 4 – 24 h.</li>
 
place plates in 3 % CO2) for 4 – 24 h.</li>
 
<li>Spot 200 μL (about 10-15 μL drops) on a sterile filter (Whatman Nuclepore Track-Etch
 
<li>Spot 200 μL (about 10-15 μL drops) on a sterile filter (Whatman Nuclepore Track-Etch
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<ul>
 
<ul>
 
<li> UTEX 2973 culture was inoculated at OD 0.1</li>
 
<li> UTEX 2973 culture was inoculated at OD 0.1</li>
<li> When UTEX 2973 culture was at OD ~0.3, cultures of prK2013 and HB101 were inoculated from
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<li> When UTEX 2973 culture was at OD ~0.3, cultures of prK2013 and HB101 were inoculated
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from
 
“overnight cultures” to OD 0.1</li>
 
“overnight cultures” to OD 0.1</li>
 
<li> When UTEX 2973 culture was at OD 0.6-0.8 the conjugation was started:</li>
 
<li> When UTEX 2973 culture was at OD 0.6-0.8 the conjugation was started:</li>
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</ol>
 
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Well-plate cultivation
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<u>Well-plate cultivation</u>
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<br>
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<ol>
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<li>inoculate colony of UDAR 4787 into liquid media in Volume of 1 mL + 0.5 μL Spec. incubate
 +
(24-48h, 42 ˙C, 130 rpm, 5% CO<sub>2</sub>, 500 μE)</li>
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<li>inoculate row A from 24-wellplate with preculture to OD<sub>730</sub>= 0.1</li>
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<li>inoculate B6 with UDAR as blank</li>
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<li>when OD reaches 0.6 inoculate row A to row C and D to OD = 0.1.</li>
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<li>well B6 to well B4+5</li>
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<u>Well-plate cultivation</u>
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<br>
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<ol>
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<li>inoculate colony of UDAR 4787 into liquid media in Volume of 1 mL + 0.5 μL Spec. incubate
+
(24-48h, 42 ˙C, 130 rpm, 5% CO<sub>2</sub>, 500 μE)</li>
+
<li>inoculate row A from 24-wellplate with preculture to OD<sub>730</sub>= 0.1</li>
+
<li>inoculate B6 with UDAR as blank</li>
+
<li>when OD reaches 0.6 inoculate row A to row C and D to OD = 0.1.</li>
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<li>well B6 to well B4+5</li>
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Revision as of 15:22, 21 October 2019

E X P E R I M E N T S


"When you're experimenting you have to try so many things before you choose what you want, and you may go days getting nothing but exhaustion."
- Fred Astaire

P R O T O C O L S


All the protocols used in our project are listed here.

L A B B O O K S


Our labbook entrys.

A U T O M A T I O N
P R O T O C O L S


The protocols of the Automation Lab can be found here.