Team:TU Darmstadt/protocols/Bacterial cell culture

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<!-- Bacterial cell culture -->
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<a href="https://2013.igem.org/Team:TU_Darmstadt/labbook">
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</a>
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<a href="https://2013.igem.org/Team:TU_Darmstadt/materials">
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<font size="8" color="#F0F8FF" face="Arial regular">Materials |</font>
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<a href="https://2013.igem.org/Team:TU_Darmstadt/protocols">
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<font size="8" color="#F0F8FF" face="Arial regular">Protocols</font>
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<h2><font size="6" color="#F0F8FF" face="Arial regular"> Bacterial cell culture </font></h2>
<h2><font size="6" color="#F0F8FF" face="Arial regular"> Bacterial cell culture </font></h2>
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<B> Materials<br></B></font></p>
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<B> Materials<br></B>
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<br>
<br>
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<B> Equipment<br></B>
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<B>Equipment<br></B>
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Bunsen burner<br>
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<div align="left" style="margin-left:60px; margin-right:50px">
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Pipettes with pleus ball<br>
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<ul>
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Micropipettes with sterile tips<br>
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<li class=list1>- Bunsen burner</li>
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Flow bench<br>
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<li class=list1>- Pipettes with peleus ball</li>
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<li class=list1>- Micropipettes with sterile tips</li>
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<li class=list1>- Flow bench</li>
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<br>
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<B> Chemicals & consumables <br></B>
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<B>Chemicals & consumables<br></B>
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Culture tubes with metal caps<br>
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Growth medium (LB, DYT or SOC)<br>
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Parafilm<br>
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<li class=list1>- Culture tubes with metal caps</li>
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Autoclaved glass pipette tubes<br>
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<li class=list1>- Growth medium: <a href="https://2013.igem.org/Team:TU_Darmstadt/materials/Media"> Media</a></li>
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<li class=list1>- Parafilm</li>
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<li class=list1>- Autoclaved glass pipette tubes</li>
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<B> Procedure<br></B>
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Starting culture: under sterile conditions add about 5mL (two fingers high) of medium to a culture tube and insert the picked colony.
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<B> Procedure<br></B></font></p><br>
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Step by step:
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Starting culture: Under sterile conditions add about 5mL (two fingers high) of medium to a culture tube and insert the picked colony.<br>
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<br>
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<li>Cultivate the stock on agar plate e.g. until colonies grow (incubation usually at 37&deg;C)</li>
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1. Cultivate the stock on agar plate e.g. until colonies grow (incubation usually at 37&deg;C)<br>
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<li>Flame a glass pipette, open the bottle of medium and flame the mouth, measure out the amount you need to fill    your tubes, flame the cap and recap the bottle as quickly as possible.</li>
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2. Flame a glass pipette, open the bottle of medium and flame the mouth, measure out the amount you need to fill    your tubes, flame the cap and recap the bottle as quickly as possible<br>
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<li>Remove the tube cap, flame the top of the culture tube, pipette in 5 ml, flame the top of the tube, and cap it  
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3. Remove the tube cap, flame the top of the culture tube, pipette in 5 ml, flame the top of the tube, and cap it  
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Pick a single colony (to asure the cells are from the same single clonal population) and transfer it to the medium
Pick a single colony (to asure the cells are from the same single clonal population) and transfer it to the medium
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by tapping a small (0.1 &mu;l) pipette tip (held on a pipette) on the surface of the plate.  Uncap a tube, flame the top, tip the tube so as to transfer cells from the pipette tip to the surface of the media without touching the inside of the tube with the non-sterile portion of the pipetter, flame, cap.  
+
by tapping a small (0.1 &mu;l) pipette tip (held on a pipette) on the surface of the plate.  Uncap a tube, flame the top, tip the tube so as to transfer cells from the pipette tip to the surface of the media without touching the inside of the tube with the non-sterile portion of the pipetter, flame, cap.</li>
-
4. Pipette the desired amount of antibiotic into each tube along the wall. Do not put the non-sterile part of the pipette inside the tube and use a new tip for each tube.<br>
+
<li>Pipette the desired amount of antibiotic into each tube along the wall. Do not put the non-sterile part of the pipette inside the tube and use a new tip for each tube.</li>
-
5. Vortex each tube for 1-2 seconds to mix well.<br>
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<li>Vortex each tube for 1-2 seconds to mix well.</li>
-
6. Take the tubes to incubat (usually at 37&deg;C) in an incubator or warm room. <br>
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<li>Take the tubes to incubat (usually at 37&deg;C) in an incubator or warm room.</li>
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7. Wait overnight or until your cells have reached the desired concentration.<br>
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<li>Wait overnight or until your cells have reached the desired concentration.</li>
 +
</ol>
 +
</div>
 +
</font></p>
<br>
<br>
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<center>
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-
<B>References<br>
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<h2><font size="6" color="#F0F8FF" face="Arial regular">References</font></h2>
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http://openwetware.org/wiki/Bacterial_cell_culture
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<font size="3" color="#F0F8FF" face="Arial regular">
 +
<ol>
 +
<li style="margin-left:15px; margin-right:50px; text-align:justify">http://openwetware.org/wiki/Bacterial_cell_culture</li>
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</ol>
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</font>

Latest revision as of 00:24, 5 October 2013







Lab book | Materials | Protocols

Bacterial cell culture

Materials


Equipment

  • - Bunsen burner
  • - Pipettes with peleus ball
  • - Micropipettes with sterile tips
  • - Flow bench


Chemicals & consumables

  • - Culture tubes with metal caps
  • - Growth medium: Media
  • - Parafilm
  • - Autoclaved glass pipette tubes


Procedure


Starting culture: Under sterile conditions add about 5mL (two fingers high) of medium to a culture tube and insert the picked colony.

  1. Cultivate the stock on agar plate e.g. until colonies grow (incubation usually at 37°C)
  2. Flame a glass pipette, open the bottle of medium and flame the mouth, measure out the amount you need to fill your tubes, flame the cap and recap the bottle as quickly as possible.
  3. Remove the tube cap, flame the top of the culture tube, pipette in 5 ml, flame the top of the tube, and cap it Pick a single colony (to asure the cells are from the same single clonal population) and transfer it to the medium by tapping a small (0.1 μl) pipette tip (held on a pipette) on the surface of the plate. Uncap a tube, flame the top, tip the tube so as to transfer cells from the pipette tip to the surface of the media without touching the inside of the tube with the non-sterile portion of the pipetter, flame, cap.
  4. Pipette the desired amount of antibiotic into each tube along the wall. Do not put the non-sterile part of the pipette inside the tube and use a new tip for each tube.
  5. Vortex each tube for 1-2 seconds to mix well.
  6. Take the tubes to incubat (usually at 37°C) in an incubator or warm room.
  7. Wait overnight or until your cells have reached the desired concentration.


References

  1. http://openwetware.org/wiki/Bacterial_cell_culture