Difference between revisions of "Team:DTU-Denmark/Experiments"

Revision as of 16:56, 4 October 2018

Experiments

Synthlab protocols

DNA from IDT will typically be delivered in a white flaky substance, which need to be resuspended, before the DNA is ready for use

Materials

Table centrifuge
EB/TE buffer
Genes/Primers from IDT or other DNA provider

Procedure

Quickly spin the DNA down in the table centrifuge
Calculate the amount of EB buffer need to dilute the gblocks to a desired concentration. Important: gene fragments and primeres are not diluted to the same concentration: The concentration of gene fragments is usually 25 ng/μL and for primers it is 100 μM.
Genes/Primers from IDT or other DNA provider
- DNA from IDT usually comes in dried flakes of 500 or 1000 ng of DNA. To achieve the desired concentration (usually 25 ng/μL) the needed amount of EB buffer is 40 μL (for 1000 ng samples) or 20 μL (for 500 ng samples)
- In order to calculate the the molar amount of primer, use the NEB calculator
Add the calculated amount of EB buffer
Store the resuspended DNA at -20°C

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Mycolab protocols

Basic protocol on plating of the fungi.

Materials

Agar plates with media of interest
Sterile toothpicks

Procedure

Plating using mycelia

Open the plate containing the mycelia from the species of interest
With a sterile toothpick, scratch the surface of the mycelia.
Spike the new agar plate with the toothpick.
Repeat steps 1-3 times. Three inoculation points should be made in the agar making forming a triangle.
Put the plate into a plastic growth bag.
Place growing bag into the incubator.

Plating using spores

Touch the sterile tooth pick in the spore suspension.
Spike the new agar plate with the toothpick.
Repeat steps 1-3 times. Three inoculation points should be made in the agar making forming a triangle.
Put the plate into a plastic growth bag.
Place growing bag into the incubator.

Minimal media used for protoplastation of A. oryzae. This is for 1 L of media.

Materials

50 mL D-glucose
50 mL Nitrate salts
1 mL Trace elements
1 mL Thiamine
20 g Agar (SO.BI.GEL)

Procedure

Mix

Mix in a blue cap flask.
Add water until the volume is 1 L.
Autoclave.

Minimal medium: Schizophyllum commune SMM agar (1L) needed for S.commune plates

Materials

Glucose - 20g
Monopotassium phosphate KH₂PO₄ - 0.46g
Potassium phosphate dibasic K₂HPO₄ 3H₂O - 1.28g
Magnesium sulfate MgSO₄ 7H₂O - 0.5g
Trace elements solution - 1ml
FeCl₃ solution - 1ml
L- Asparagin - 1.5g
Agar - 20g
Thiamine (10mg/100ml) - 1.2ml

Procedure

Preparation of the media

Weigh and add the required solid components (except agar)
Add the required liquid components in a bottle
Dissolve in demineralized water until the total volume is 900ml
Stir the liquid using a magnet (no pH adjustment is required)
Add the required quantity of agar
Add demineralized water until the desired total volume (1L)
Autoclave
After sterilization add 1.2 ml of filter sterilized thiamine

@@ Line 259: / Line 259: @@
 <ul>
    <li><p>Glucose - 20g</p></li>
-  <li><p>Monopotassium phosphate KH<sub>2<\sub>PO<sub>4</sub> - 0.46g</p></li>
+  <li><p>Monopotassium phosphate KH<sub>2</sub>PO<sub>4</sub> - 0.46g</p></li>
-<li><p>Potassium phosphate dibasic K<sub>2<\sub>HPO<sub>4<\sub>  3H<sub>2<\sub>O - 1.28g</p></li>
+<li><p>Potassium phosphate dibasic K<sub>2</sub>HPO<sub>4</sub>  3H<sub>2</sub>O - 1.28g</p></li>
-  <li><p>Magnesium sulfate MgSO<sub>4<\sub>  7H<sub>2<\sub>O - 0.5g</p></li>
+  <li><p>Magnesium sulfate MgSO<sub>4</sub>  7H<sub>2</sub>O - 0.5g</p></li>
 <li><p>Trace elements solution - 1ml </p></li>
-  <li><p>FeCl<sub>3<\sub> solution - 1ml</p></li>
+  <li><p>FeCl<sub>3</sub> solution - 1ml</p></li>
 <li><p>L- Asparagin - 1.5g</p></li>
   <li><p>Agar - 20g</p></li>