Team:Aachen/Notebook/Protocols/detection

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(Measurement of Fluorescence)
(Measurement of Fluorescence)
 
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   <li style="width:106px;margin-left: 12px;margin-right: 12px;" >
     <a class="menulink" href="https://2014.igem.org/Team:Aachen/Notebook/Protocols/Culture_medium_and_conditions" style="color:black">
     <a class="menulink" href="https://2014.igem.org/Team:Aachen/Notebook/Protocols/Culture_medium_and_conditions" style="color:black">
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     <div class="menusmall-item menusmall-info" style="height:100px; width: 100px;" ><div class="menukachel" style="top: 10%; font-size: 14px;">Culture Media &<br/>Culture Conditions</div></div>
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     <div class="menusmall-item menusmall-info" style="height:100px; width: 100px;" ><div class="menukachel" style="top: 10%; font-size: 14px;">Culture Media</div></div>
     <div class="menusmall-item menusmall-img" style="background: url(https://static.igem.org/mediawiki/2014/1/10/Aachen_14-10-13_Yellow_Flask_iNB.png); norepeat scroll 0% 0% transparent; background-size:100%; height:100px; width: 100px;">
     <div class="menusmall-item menusmall-img" style="background: url(https://static.igem.org/mediawiki/2014/1/10/Aachen_14-10-13_Yellow_Flask_iNB.png); norepeat scroll 0% 0% transparent; background-size:100%; height:100px; width: 100px;">
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= 2D Detection of IPTG and HSL =
= 2D Detection of IPTG and HSL =
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The protocol for the chip production was developed by this year's iGEM Team Aachen with [https://2014.igem.org/User:Aschechtel Anna] as driving force and person in charge. A lot of parameters were tested and the final protocol for the production of the sensor chips the way there were used for detection in the project is published below.
+
The method of the chip production was developed by this year's iGEM Team Aachen with [https://2014.igem.org/User:Aschechtel Anna] as driving force and person in charge. A lot of parameters were tested and the final protocol for the production of the sensor chips the way there were used for detection in the project is published below.
== Chip Production ==
== Chip Production ==
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'''Cell Preparation'''
'''Cell Preparation'''
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# over night culture of sensor cells (50&nbsp;mL in a 250&nbsp;mL flask with) max. 16&nbsp;h
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# over night culture of sensor cells (50&nbsp;ml in a 250&nbsp;ml flask with) max. 16&nbsp;h
-
# centrifuge all 50&nbsp;mL by 3000&nbsp;g for 10 min at RT (21&nbsp;°C).
+
# centrifuge all 50&nbsp;ml by 3000&nbsp;g for 10&nbsp;min at RT (21°C).
# discard the supernatant
# discard the supernatant
-
# re-suspend the pellet in 1&nbsp;mL tempered (~21&nbsp;°C) LB-medium.
+
# re-suspend the pellet in 1&nbsp;mL tempered (~21°C) LB-medium.
'''Agar Preparation'''
'''Agar Preparation'''
-
# autoclave 50&nbsp;mL medium with 1.5&nbsp;%&nbsp;(w/v) agarose (has to be multiplied with the number of chips prepared).
+
# autoclave 50&nbsp;ml medium with 1.5%(w/v) agarose (has to be multiplied with the number of chips prepared).
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# cool it down to 45&nbsp;°C in a water bath.
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# cool it down to 45°C in a water bath.
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# mix the cooled medium with the cells by inverting gently.
# mix the cooled medium with the cells by inverting gently.
-
# pour it in the chip form, avoiding bubble formation (!).
+
# pour it in the chip mold, avoiding bubble formation (!).
# wait for approximately 20 min until the agar has solidified.
# wait for approximately 20 min until the agar has solidified.
# cut out the chips with a scalpel.
# cut out the chips with a scalpel.
# put two chips into a labeled petri dish and store additional 4 chips in labeled petri dishs in the refrigerator.
# put two chips into a labeled petri dish and store additional 4 chips in labeled petri dishs in the refrigerator.
-
# incubate two chips for 1&nbsp;h at 37&nbsp;°C prior to induction.
+
# incubate two chips for 1&nbsp;h at 37°C prior to induction.
 +
 
<center>
<center>
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{{Team:Aachen/Figure|Aachen 14-10-09 flowsheet chip manufacturingV8 ipo.png|title=Sensor-chip manufacturing|subtitle=Scheme illustrating the work flow during chip production.|width=1000px}}
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{{Team:Aachen/Figure|Aachen 14-10-09 flowsheet chip manufacturingV8 ipo.png|title=Sensor-chip manufacturing|subtitle=Scheme illustrating the work flow during chip production. For the production steps see above.|width=1000px}}
</center>
</center>
== Measurement of Fluorescence ==
== Measurement of Fluorescence ==
-
For the measurement of fluorescence in our sensor chips we used three different methods. The first was done by using our measurement device [https://2014.igem.org/Team:Aachen/Project/Measurement_Device WatsOn]. You can read even more about building your own WatsOn [https://2014.igem.org/Team:Aachen/Notebook/Engineering/WatsOn here]. Secondly we used the Platereader [http://www.biotek.com/products/microplate_detection/synergymx_monochromator_based_multimode_microplate_reader.html Synergy Mx from BioTek]. We put the sensor chips into the lid of a normal well plate and then measured GFP with an excitation of 496&nbsp;±&nbsp;9&nbsp;nm and an emission of 516&nbsp;±&nbsp;9&nbsp;nm and iLOV with an excitation of 450&nbsp;±&nbsp;9&nbsp;nm and emission of 495&nbsp;±&nbsp;9&nbsp;nm. Thirdly we used the ??? Geldoc with ??? settings.
+
For measurement of a fluorescence response in our sensor chips we used three different methods.
 +
 
 +
'''First''', the '''Gel Doc™ XR+''' (BIO-RAD) was used, exciting with UV light for an exposure time of 1&nbsp;s.
 +
 
 +
'''Second''', we used our own device [https://2014.igem.org/Team:Aachen/Project/Measurement_Device '''''WatsOn'''''] with blue light for excitation (450 or 480&nbsp;nm) and special filters infront of the camera for selecting the appropriate emission spectrum. You can read even more about building your own ''WatsOn'' [https://2014.igem.org/Team:Aachen/Notebook/Engineering/WatsOn here].
 +
 
 +
'''Third''', we used the '''Synergy Mx microplate reader''' (BioTek), putting the sensor chips into the lid of a common clear well plate. GFP was measured with an excitation of 496&nbsp;±&nbsp;9&nbsp;nm and an emission of 516&nbsp;±&nbsp;9&nbsp;nm and iLOV with an excitation of 450&nbsp;±&nbsp;9&nbsp;nm and emission of 495&nbsp;±&nbsp;9&nbsp;nm.
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   <li style="width:106px;margin-left: 12px;margin-right: 12px;" >
   <li style="width:106px;margin-left: 12px;margin-right: 12px;" >
     <a class="menulink" href="https://2014.igem.org/Team:Aachen/Notebook/Protocols/Culture_medium_and_conditions" style="color:black">
     <a class="menulink" href="https://2014.igem.org/Team:Aachen/Notebook/Protocols/Culture_medium_and_conditions" style="color:black">
-
     <div class="menusmall-item menusmall-info" style="height:100px; width: 100px;" ><div class="menukachel" style="top: 10%; font-size: 14px;">Culture Media &<br/>Culture Conditions</div></div>
+
     <div class="menusmall-item menusmall-info" style="height:100px; width: 100px;" ><div class="menukachel" style="top: 10%; font-size: 14px;">Culture Media</div></div>
     <div class="menusmall-item menusmall-img" style="background: url(https://static.igem.org/mediawiki/2014/1/10/Aachen_14-10-13_Yellow_Flask_iNB.png); norepeat scroll 0% 0% transparent; background-size:100%; height:100px; width: 100px;">
     <div class="menusmall-item menusmall-img" style="background: url(https://static.igem.org/mediawiki/2014/1/10/Aachen_14-10-13_Yellow_Flask_iNB.png); norepeat scroll 0% 0% transparent; background-size:100%; height:100px; width: 100px;">
     </div>
     </div>

Latest revision as of 21:23, 17 October 2014

2D Detection of IPTG and HSL

The method of the chip production was developed by this year's iGEM Team Aachen with Anna as driving force and person in charge. A lot of parameters were tested and the final protocol for the production of the sensor chips the way there were used for detection in the project is published below.

Chip Production

Cell Preparation

  1. over night culture of sensor cells (50 ml in a 250 ml flask with) max. 16 h
  2. centrifuge all 50 ml by 3000 g for 10 min at RT (21°C).
  3. discard the supernatant
  4. re-suspend the pellet in 1 mL tempered (~21°C) LB-medium.


Agar Preparation

  1. autoclave 50 ml medium with 1.5%(w/v) agarose (has to be multiplied with the number of chips prepared).
  2. cool it down to 45°C in a water bath.


Chip Preparation

  1. mix the cooled medium with the cells by inverting gently.
  2. pour it in the chip mold, avoiding bubble formation (!).
  3. wait for approximately 20 min until the agar has solidified.
  4. cut out the chips with a scalpel.
  5. put two chips into a labeled petri dish and store additional 4 chips in labeled petri dishs in the refrigerator.
  6. incubate two chips for 1 h at 37°C prior to induction.


Aachen 14-10-09 flowsheet chip manufacturingV8 ipo.png
Sensor-chip manufacturing
Scheme illustrating the work flow during chip production. For the production steps see above.

Measurement of Fluorescence

For measurement of a fluorescence response in our sensor chips we used three different methods.

First, the Gel Doc™ XR+ (BIO-RAD) was used, exciting with UV light for an exposure time of 1 s.

Second, we used our own device WatsOn with blue light for excitation (450 or 480 nm) and special filters infront of the camera for selecting the appropriate emission spectrum. You can read even more about building your own WatsOn here.

Third, we used the Synergy Mx microplate reader (BioTek), putting the sensor chips into the lid of a common clear well plate. GFP was measured with an excitation of 496 ± 9 nm and an emission of 516 ± 9 nm and iLOV with an excitation of 450 ± 9 nm and emission of 495 ± 9 nm.