Difference between revisions of "Team:SJTU-BioX-Shanghai/Protocol"

Revision as of 08:23, 30 October 2017

Protocol

PCR

Materials:

Buffer
Mg²⁺
dNTP
Template
F/R-primer
DNA enzyme

Methods:

Combination of all reagents

Name of reagent	volume (μl)
Buffer	2
Mg²⁺	2
Template	20 ng for plasmid or 200 ng for genome
F/R-primer	0.6 for each
Enzyme	0.4
Sterile Water	make reaction up to 20μ in total

Set the PCR machine to run the following steps:

Stage	Temperature (℃)	Time
initial denaturation	94	2 min
	94 (denaturation)	15 seconds
30 cycles	40-55 (annealing)	30 seconds
	68 (extension)	30 seconds per bp
Final extension	68	7 min
Incubate	12	Infinite

Restriction Digestion

Materials:

Restriction Enzyme: Fisher FastDigest Restriction Enzyme
Green Buffer
DNA samplesr
Sterile Water

Methods:

Note: the components listed below are for double digestion!

Component	volume (μl)
Green Buffer	2
DNA sample	600 ng for plasmid or up to 200 ng for PCR production
Template	20 ng for plasmid or 200 ng for genome
Restriction Enzyme	1 for each
Sterile Water	make reaction up to 20μ in total

Set up the reaction following the above table and incubate at 37℃ for 15-30 min and do the gel electrophoresis or purification later

Ligation

Materials:

T4 DNA Ligase
T4 DNA Ligase Buffer
Vector Plasmid
Insert DNA
Sterile Water

Methods:

Component	volume or mass
T4 DNA Ligase Buffer	2 μ
Vector Plasmid	50 ng
Insert DNA	require molar ratio of 3:1 to 7:1 (insert:vector)
T4 DNA Ligase	0.2 μ
Sterile Water	make reaction up to 20μ in total

Make the reaction and incubate at room temperature for 4-6 hours

Note: for how to calculate volumes of vector and insert DNA, we highly recommend NEBbioCalculator

DNA Gel Electrophoresis

Materials:

Agarose
TBE Buffer
Gel board
EB
DNA×10 or×6 Loading Buffer
Electrophoresis tank
sample
marker 2000 or 15000

Methods:

Make a 1.0%-1.5% Agarose gel according to the volume of your gel board (eg. add 0.45g Agarose in 30ml TBE if choose a concentration of 1.5%)
Heat the container with the mixture until it is complete dissolved. When the solution starts boiling, stop heating, shake the container until materials mix well and heat again until the mixture become clear
Wait until the solution cools down to 50℃,add 0.01% EB (eg. 3μin 30ml) or non-poisonous dyes instead
Pour the solution into a gel board and insert the comb
Set the gel at room temperature and wait until it completely solidifies
Remove the comb and transfer the gel to the electrophoresis tank
Add samples into pores with 40% DNA Loading Buffer (eg. 2μLoading Buffer in 5μDNA sample)
Run the gel for 20 min at 100V, 100mA

Transformation

Materials:

LB broth
Ice
Selection plates with corresponding antibiotics.

Methods:

Put 50µL competent E. coli cells on ice for 10 minutes
Add 20 µl DNA from a ligation reaction mix or 10-100 ng plasmid
Incubate the mixture on ice for 30 minutes
Heat shock at exactly 42°C for exactly 45 seconds
Place on ice for 3 minutes
add the mixture into 500 µL LB broth
Incubate at 37°C and 200-250 rpm for one hour
For ligation reaction DNA: 500 µl of each transformation reaction onto a selection plate. For known plasmid: 100-200 µL of each transformation reaction onto a selection plate
Incubate overnight at 37°C with plates upside down.

Purification and Gel Extraction & Plasmid Extraction

Purification of PCR or restriction products was performed according to the OMEGA Cycle Pure Kit D6492.

Gel Extraction was performed according to the OMEGA Gel Extraction Kit D2500.

Plasmid Extraction was performed according to the BIOMIGA Plasmid Miniprep Kit.

Cotransformation

Characterization

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                          <p>Make the reaction and incubate at room temperature for 4-6 hours</p>
                          <p>Note: for how to calculate volumes of vector and insert DNA, we highly recommend <a target="_blank" href="http://nebiocalculator.neb.com/#!/ligation">NEBbioCalculator</a></p>
-                        <p>Sterile Water</p>
                          <div class="my-title h5-my-responsive" id="section4">DNA Gel Electrophoresis</div>
                          <p class="my-title2">Materials:</p>
@@ Line 325: / Line 325: @@
                              <li>add the mixture into 500 µL LB broth</li>
                              <li>Incubate at 37°C and 200-250 rpm for one hour</li>
-                             <li>For ligation reaction DNA: 500 µl of each transformation reaction onto a selection plate.
+                             <li>For ligation reaction DNA: 500 µl of each transformation reaction onto a selection plate. For known plasmid: 100-200 µL of each transformation reaction onto a selection plate
-                                For known plasmid: 100-200 µL of each transformation reaction onto a selection plate
+                            </li>
-                                </li>
                              <li>Incubate overnight at 37°C with plates upside down.</li>
                          </ol>
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