Difference between revisions of "Team:Alverno CA/MakingtheAgaroseGel"

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<p>Ingredients/Materials: *</p>
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<center><p>Ingredients/Materials: *</p>
 
<p>- 0.6g agarose</p>
 
<p>- 0.6g agarose</p>
 
<p>- 50mL TBE 1x</p>
 
<p>- 50mL TBE 1x</p>
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<p>      6. Set machine to 175V and for 20 minutes. Make sure bubbles are appearing!</p>
 
<p>      6. Set machine to 175V and for 20 minutes. Make sure bubbles are appearing!</p>
 
<p>      7. After running place gel onto transilluminator (must be off) in glove box. Place box over it with hole and then place iPad above it and set to either video or time-lapse. Then turn on transilluminator within closed glove box while videotaping. </p>
 
<p>      7. After running place gel onto transilluminator (must be off) in glove box. Place box over it with hole and then place iPad above it and set to either video or time-lapse. Then turn on transilluminator within closed glove box while videotaping. </p>
<p>      8. Results can now be analyzed. </p>
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<p>      8. Results can now be analyzed. </p></center>
 
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Revision as of 00:05, 6 October 2016

Making the Agarose Gel

Experiment & Protocol

Alverno iGEM Logo

Making the Agarose Gel

*Note: Pipettes are needed.

Ingredients/Materials: *

- 0.6g agarose

- 50mL TBE 1x

- 5μL SYBRsafe / 2.5μL EcoStain (light- and heat-sensitive)

- 250mL conical flask

- scale

- Microwave

- Gel mold

Directions:

1. Weigh 0.6g of agarose into flask.

2. Add 50mL of TBE 1x Buffer

3. Microwave agarose solution until dissolved for 1 min (take out halfway to swirl)

(If the liquid looks distorted, agarose solution need to be microwaved more)

4. Cool slightly and add SYBRsafe or EcoStain

5. Pour gel into mold and put the combs into their spots

6. Cool until solidified.

Gel Electrophoresis & Screening the gel

Ingredients/Materials: *

- TBE 1x Buffer

- agarose gel (w/ right number of wells)

- DNA reaction (either parts=PUCTV, or PCR check for GG plasmids)

- purple loading dye

- Gel box

Directions:

1. Place agarose gel into gel box with wells on negative side.

2. Fill up gel box up with TBE 1x Buffer up to line or at least above gel.

3. Pipette 6ul of 2-log ladder on side lanes (or given wells).

4. Pipette 1ul of purple loading dye on parafilm. Then pipette 5ul of DNA reaction and mix with loading dye on parafilm. (*For PCR Check: Directly pipette 2ul of purple loading dye into 10ul of PCR Check Reaction in microfuge tube)

5. Set to 6ul and pipette 6ul of mixed reaction with loading dye into selected wells according to drawn diagram. See gel picture.

6. Set machine to 175V and for 20 minutes. Make sure bubbles are appearing!

7. After running place gel onto transilluminator (must be off) in glove box. Place box over it with hole and then place iPad above it and set to either video or time-lapse. Then turn on transilluminator within closed glove box while videotaping.

8. Results can now be analyzed.