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Team:Paris Saclay/Protocols/BioBrick Assembly
From 2014.igem.org
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## Make a gel '''0.8%''' agarose | ## Make a gel '''0.8%''' agarose | ||
## Use xxx of BET concentration | ## Use xxx of BET concentration | ||
| - | ## Use a box with a | + | ## Use a box with a long height and a double case for the DNA. |
## Run the gel at 100V for one hour | ## Run the gel at 100V for one hour | ||
# minimal exposure of UV light | # minimal exposure of UV light | ||
# mass of the ependorf (before / after) | # mass of the ependorf (before / after) | ||
| + | |||
| + | ''<u>Note:</u> Minimize UV exposure time to avoid damaging the DNA.'' | ||
====DNA extration from agarose gels==== | ====DNA extration from agarose gels==== | ||
| - | + | # Excise DNA fragment / solubilize gel slice | |
| - | + | ## Determine the weight of the (Eppendorf) tube prior to use. | |
| + | ## Put the DNA fragment with a minimal agarose gel into the tube. | ||
| + | ## Determine the weight of the gel slice by the difference of the tube's weight. | ||
| + | ## For each 100 mg of agarose gel < 2% add 200 μl Buffer NTI. | ||
| + | ## Incubate sample for 5-10 min at 50°C. | ||
| + | ## Vortex the sample briefly every 2-3 min until the gel slice is completely dissolved. | ||
| + | # Bind DNA | ||
| + | ## Place a NucleSpin Gel and PCR Clean-up Column into a Collection Tube and load up to 700 μl sample. | ||
| + | ## Centrifuge for 30 seconds at 11,000 x g. Discard flow-through. | ||
| + | ## Load remaining sample if necessary and repeat the centrifugation step. | ||
| + | # Wash silica membrane | ||
| + | ## Add 700 μl Buffer NT3 to the column. Centrifuge for 30 s at 11,000 x g. Discard flow-through. | ||
| + | # Dry silica membrane | ||
| + | ## Centrifuge for 1 min at 11,000 x g to remove Buffer NT3 completely. | ||
| + | # Elute DNA | ||
| + | ## Place the column into a new 1.5 ml micro centrifuge tube. Add 15-30 μl Buffer NE and incubate at room temperature (18-25 °C) for 1 min. | ||
| + | ## Centrifuge for 1 min at 11,000 x g. | ||
====Ligation==== | ====Ligation==== | ||
Revision as of 08:16, 5 August 2014
Contents |
BioBrick Assembly
This protocol is based on the original [http://parts.igem.org/Help:Assembly/3A_Assembly 3A Assembly] from iGEM. We modified it to a assembly that places the core of one BioBrick - here called Part A - into another BioBrick - here called Part B.
TODO: Process illustration [Format I and Format II]
Procedure
Enzymes
Note: Manipulate the enzymes with a proper subzero temperature support.
Part A:
- Enzyme A: EcoRI
- Enzyme B: SpeI
Part B with Format I (Part B placed after Part A):
- Enzyme A: EcoRI
- Enzyme B: XbaI
Part B with Format II (Part B placed before Part A):
- Enzyme A: SpeI
- Enzyme B: PstI
Digest reaction
- Take a 1.5ml microcentrifuge tube (Eppendorf) and put:
- xμl of H20 milliQ (complement)
- 5μl of buffer (Fast Digest Buffer 10x)
- xμl of Part A DNA
- 1μl of Enzyme A
- 1μl of Enzyme B
- Repeat step 1 with Part B
- Mix gently both tubes
- Incubate at 37°C for one hour
- Store Part B at -20°C.
Segregate process
- part A
- Follow the Electrophoresis Protocol with the following parameters:
- Make a gel 0.8% agarose
- Use xxx of BET concentration
- Use a box with a long height and a double case for the DNA.
- Run the gel at 100V for one hour
- minimal exposure of UV light
- mass of the ependorf (before / after)
Note: Minimize UV exposure time to avoid damaging the DNA.
DNA extration from agarose gels
- Excise DNA fragment / solubilize gel slice
- Determine the weight of the (Eppendorf) tube prior to use.
- Put the DNA fragment with a minimal agarose gel into the tube.
- Determine the weight of the gel slice by the difference of the tube's weight.
- For each 100 mg of agarose gel < 2% add 200 μl Buffer NTI.
- Incubate sample for 5-10 min at 50°C.
- Vortex the sample briefly every 2-3 min until the gel slice is completely dissolved.
- Bind DNA
- Place a NucleSpin Gel and PCR Clean-up Column into a Collection Tube and load up to 700 μl sample.
- Centrifuge for 30 seconds at 11,000 x g. Discard flow-through.
- Load remaining sample if necessary and repeat the centrifugation step.
- Wash silica membrane
- Add 700 μl Buffer NT3 to the column. Centrifuge for 30 s at 11,000 x g. Discard flow-through.
- Dry silica membrane
- Centrifuge for 1 min at 11,000 x g to remove Buffer NT3 completely.
- Elute DNA
- Place the column into a new 1.5 ml micro centrifuge tube. Add 15-30 μl Buffer NE and incubate at room temperature (18-25 °C) for 1 min.
- Centrifuge for 1 min at 11,000 x g.
