Difference between revisions of "Projet Sylvan"

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(Protocols)
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== Etc... ==
 
== Etc... ==
 +
 +
<br>
  
 
= Protocols =
 
= Protocols =
  
== LB Agar ==
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== Growth Media ==
 +
=== LB Agar ===
  
 
More details [https://en.wikipedia.org/wiki/Lysogeny_broth here].<br>
 
More details [https://en.wikipedia.org/wiki/Lysogeny_broth here].<br>
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* add dH2O to 500mL
 
* add dH2O to 500mL
  
<br>
 
Note: If your lab has pre-mixed LB agar powder, use the suggested amount instead of the other dry ingredients above.
 
 
<br>
 
<br>
 
Swirl to mix - the contents do not have to be completely in solution, but any powder left on the sides of the flask will caramelize on the glass during autoclaving.
 
Swirl to mix - the contents do not have to be completely in solution, but any powder left on the sides of the flask will caramelize on the glass during autoclaving.
 
<br>
 
<br>
Cover the top of the flask with aluminum foil and label with autoclave tape.
+
 
 +
Cover the top of the flask with aluminum foil or with a lid
 +
'''Do not close tightly as it may explode!'''
 +
 
 +
Label with autoclave tape (if you have some).
 +
 
 
<br>
 
<br>
Autoclave on the liquid setting for 20 minutes or according to your autoclave's specifications.
+
Autoclave on the liquid setting for 20 minutes (be aware that the full autoclave's cycle takes about 3 hours to complete)
 +
 
 
<br>
 
<br>
After removing the solution from the autoclave, allow the agar solution to cool to 55°C.
+
After removing the solution from the autoclave (at 75 °C), allow the agar solution to cool to 55 °C.
 +
 
 
<br>
 
<br>
Note: This can be done by placing the flask in a 55°C oven or water bath, as this will hold the temperature and it can be left unattended for some time.
+
When pouring plates, keep your bench area sterile by working in a laminar flow hood (turn it on 30 minutes before and clean with ethanol before use).
 +
 
 
<br>
 
<br>
When pouring plates, keep your bench area sterile by working near a flame or bunsen burner.
+
Pour ~ 15-20mL of LB agar in each 96mm polystyrene Petri dish.
<br>
+
 
Add the appropriate amount of desired antibiotic to the solution (500µL if you are using a 1,000x antibiotic stock) and swirl to mix.
+
<br>
+
Pour ~20mL of LB agar per 10cm polystyrene Petri dish.
+
 
<br>
 
<br>
 
Note: Pour slowly from the flask into the center of the petri dish. When the agar has spread to cover about 2/3 of the dish stop pouring and the agar should spread to cover the entire plate. You may need to tilt the plate slightly to get the agar to spread out completely. If you pour in too much, the plate will be fine, but it will reduce the number of plates you can make per batch.
 
Note: Pour slowly from the flask into the center of the petri dish. When the agar has spread to cover about 2/3 of the dish stop pouring and the agar should spread to cover the entire plate. You may need to tilt the plate slightly to get the agar to spread out completely. If you pour in too much, the plate will be fine, but it will reduce the number of plates you can make per batch.
 +
 
<br>
 
<br>
Note: If bubbles are introduced during the pouring, these can be removed by quickly passing the flame of an inverted bunsen burner over the surface of the plate. Be careful, if you leave the flame too long it will melt the petri dish. Also be careful not to burn yourself.
+
Do not place the lids on the plates before they are cold (allow them to cool for 30 minutes, until solidified), then invert the plates. Let sit for several more hours or overnight.
 +
 
 
<br>
 
<br>
Place the lids on the plates and allow them to cool for 30-60 minutes (until solidified), then invert the plates. Let sit for several more hours or overnight.
+
Label the bottom of plates with date and store in plastic bags or sealed with parafilm at 4°C.
 +
 
 
<br>
 
<br>
Label the bottom of plates with antibiotic and date and store in plastic bags or sealed with parafilm at 4°C.
+
=== Light Glucose medium ===
<br>
+
== Light Glucose medium ==
+
  
 
In 500 mL Schott Bottle:<br>
 
In 500 mL Schott Bottle:<br>
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* 8 g Agar
 
* 8 g Agar
 
* add dH2O to 500mL
 
* add dH2O to 500mL
 +
 +
Same procedure as above to make petri agar plates.

Revision as of 15:35, 14 November 2015

Goal

Etc...


Protocols

Growth Media

LB Agar

More details here.

Protocol To make 500mL of LB agar (makes about 25 LB agar plates):

Weigh out the following into a 500mL Schott Bottle:

  • 5g NaCl
  • 5g Tryptone
  • 2.5g Yeast Extract
  • 7.5g Agar
  • add dH2O to 500mL


Swirl to mix - the contents do not have to be completely in solution, but any powder left on the sides of the flask will caramelize on the glass during autoclaving.

Cover the top of the flask with aluminum foil or with a lid Do not close tightly as it may explode!

Label with autoclave tape (if you have some).


Autoclave on the liquid setting for 20 minutes (be aware that the full autoclave's cycle takes about 3 hours to complete)


After removing the solution from the autoclave (at 75 °C), allow the agar solution to cool to 55 °C.


When pouring plates, keep your bench area sterile by working in a laminar flow hood (turn it on 30 minutes before and clean with ethanol before use).


Pour ~ 15-20mL of LB agar in each 96mm polystyrene Petri dish.


Note: Pour slowly from the flask into the center of the petri dish. When the agar has spread to cover about 2/3 of the dish stop pouring and the agar should spread to cover the entire plate. You may need to tilt the plate slightly to get the agar to spread out completely. If you pour in too much, the plate will be fine, but it will reduce the number of plates you can make per batch.


Do not place the lids on the plates before they are cold (allow them to cool for 30 minutes, until solidified), then invert the plates. Let sit for several more hours or overnight.


Label the bottom of plates with date and store in plastic bags or sealed with parafilm at 4°C.


Light Glucose medium

In 500 mL Schott Bottle:

  • 2 g Glucose
  • 2 g Yeast Extract
  • 1 g NaCl
  • 8 g Agar
  • add dH2O to 500mL

Same procedure as above to make petri agar plates.