Transient transfection of Jurkat T cells

1. Culturing of cells before nucleofection. Cells should be nucleofected after reaching 70-85% confluency, higher cell densities may cause lower nucleofection efficiencies, mycoplasma contamination will negatively influence experiments results.
2. Combine the cells of interest, DNA and the appropriate cell-type specific Nucleofection Solution (Here Buffer C), and transfer to an amaxa certified cuvette (invitrogen cuvette). 1X106-5-106 cells, 1-5ug plasmid DNA in 1-5 H2O or TE, and 100 room temperature Buffer are used in this step. The quapty and the concentration of DNA used for nucleofection plays a central role for the efficiency of gene transfer. We strongly recommend the use of high quapty products for plasmid purification pke Qiagen endofree plasmid kit. The purified DNA shod be resuspended in deionised water or TE buffer with a concentration between 1-5ug/. The ration of A260;A280 shod be at least 1.8 for nucleofection
3. Insert the cuvette into the Nucleofector TM and choose the cell-type specific program. Press the start button "X". If the program is unknown, please following the recommend above. To avoid damage to the cells remove the sample from the cuvette immediately after the program has finished (display showing "OK")
4. Rinse the cuvette with cture medium and transfer the cells into the cture dish.
5. Incubate at 37°C until use.

Lipofectamine 2000 DNA Transfection Reagent Protocol

1、Seed cells to be 70–90% confluent at transfection.
2、Dilute four amounts of ppofectamine® Reagent in Opti-MEM® Medium Opti-MEM® Medium.
3、Dilute DNA in Opti-MEM® Medium.
4、Add diluted DNA to diluted ppofectamine® 2000 Reagent (1:1 ratio)
5、Incubate for 20 minutes at room temperature.
5、Add DNA-ppid complex to cells.
6、Incubate cells for 1–3 days at 37°C. Then analyze transfected cells.

Calcium Phosphate Transfection

Dissolve, in 950 ml H2O. Adjust pH to exactly 7.5 with 1N HCL, bring up to 1L with ddH2O. Filter using 0.22 micron filter. Apquot in 50 ml Falcon tubes. Store at -20℃
2M CaCl2: Filters steripze. Store in 1 ml apquots at -20℃. Stable at RT

Transfection

1. Twenty-tour hours prior to transfection, inocate 1-2×106 cells/10 cm plate in 10 ml DMEM/F12 media + 10% BCS supplemented with L-glutamine and Pen/Strep. At the time of transfection, cells shod be about 60-70% confluent
2. The following day (20-24 hours later), transfect cells. Up to 15 to 20 µg DNA can be used for one 10-cm plate. If more than one plasmid is used for transfecting the same plate, equapze DNA amounts among different plates by adding vector plasmid DNA to some plates, so that the total amount of plasmids used for each plate is the same. For transfection.
a. Prepare the following mix for 10 cm plate.
61 vL 2M CaCl2.
10ug DNA total
Add ddH2O to 500
Vortex to mix.
b. Slowly (drop-wise) add 0.5 ml of 2x HBS while typing the mixture prepared in (a)
c Drop total 1 mI of the final mix around the plate, then mix gently. Place the plate back in the incubator.
3. Twelve to 16 hours after transfection, gently aspirate the medium and add 10 ml of pre-warmed fresh medium to the plates. Try not to disturb the fine DNA-CaPO4 precipitates on the bottom of the plate
4. The following day, harvest the cells and extract protein as needed

RT-qPCR

Western blot

Transferring the protein from the gel to the membrane

1. Need 6 pieces of filter paper (11 x 14.5 cm) and 1 piece of Hybond-P PVDF membrane of the same size.
2. Hydrate Hybond-P by placing in methanol for 3 minutes and in transfer buffer for 10 min.
3. Remove gel from electrophoresis apparatus and cut to size.
4. Place gel in transfer buffer for 10 min.
5. Assemble the transfer cassette as follows (black side down): fiber pad (pre-wet in transfer buffer), filter paper (x3, pre-wet), gel (no bubbles), Hybond-P PVDF membrane (non bubbles), filter paper (x3, pre-wet) and fiber pad (pre-wet).
6. Place cassette in transfer cell (black on black).
7. Add transfer buffer to the electrophoresis tank.
8. Connect to powerpac and run at constant amps (300mA) for 90 minutes, keep the temperature at 4℃.
9. Remove membrance and, if necessary, keep hydrated in TBS in the cold room until needed.

Package the virus (For stable transfection)

1. Add three virus packed plasmids and target plasmids to a 6cm plate according to the transfection method of Lipo2000.
2. After 6 hours, replace the cell culture medium.
3. After 48 hours, the cell supernatant in the whole plate was recycled into a 15ML centrifuge tube (cell fragments may be cracked in the supernatant).
4. Centrifuge for 10 minutes at 12000rpm.
5. recycling supernatant, it can be applied directly to infect cells, or be saved in - 20 ℃

Verify upstream pathway

1. Infected jurkat T cells with the same amount of packaged viruses containing plasmids A, B and C.
2. The cells were screened for 7 days with antibiotics BSD (5ug/ml) and PURO (1ug/ml).
3. Continue to culture the cells when the cells no longer decrease.
4. Transfected the plasmid expressing GFP on the membrane into 293T cells according to the method of Lipo2000.
5. After 48 hours, remove the culture medium of 293T, and add Jurkat T cells with cell ratio 1:1 to incubate for 1 hour.
6. Recycle the incubated Jurkat T cells into one hole of the new 6-well plate, and add the unincubated Jurkat T cells in the same amount to another hole.
7. The fluorescent color of the two groups of cells is observed with a fluorescence microscope.

PCR(using Phanta Max Super-Fidepty DNA Polymerase PCR amppfication system)

Thermocycpng conditions for a Routine PCR:

Methods:
1. Prepare the reaction system in a PCR tube on ice, thaw the components and mix well. After use, put them back in -20 ℃.
2. Gently centrifuge to collect the pquid at the bottom of the tube.
3. Transfer the PCR tube to the PCR machine, set the parameters and start the thermal cycle.

Agarose Gel Electrophoresis

Methods(for a 1% Gel): 1. Place the gel tray in the appropriate position in the gel cartridge and place the comb in the correct position.
2. Measure 0.5g agarose , put it in a 250 mL Erlenmeyer flask, add 50 mL 1 x TAE buffer and mix, then put the Erlenmeyer flask in the oven and heat to boil until the agarose is completely dissolved.
3. Add 5μL GelRed to the solution.
4. Pour the solution into the gel casting tray.
5. After the gel cools to sopd, pl out the comb.
6. Place the gel in the electrophoresis chamber with enough TAE buffer.
7. Add 10×loading buffer to the sample and mix, then transfer the mixture to the well on the gel with a pipette.
8. Power on,run at 120 V for half an hour.

Gel Extraction

According to the E.Z.N.A. Gel Extraction kit
1.Perform agarose gel/ethidium bromide electrophoresis to fractionate DNA fragments. Any type or grade of agarose may be used. However, it is strongly recommended that fresh TAE buffer or TBE buffer be used as running buffer. Do not reuse running buffer as its pH will increase and reduce yields.
2.When adequate separation of bands has occurred, carefly excise the DNA fragment of interest using a wide, clean, sharp scalpel. Minimize the size of the gel spce by removing extra agarose.
3.Determine the appropriate volume of the gel spce by weighing it in a clean 1.5 mL microcentrifuge tube. Assuming a density of 1 g/mL, the volume of gel is derived as follows: a gel spce of mass 0.3 g will have a volume of 0.3 mL. 4. Add 1 volume Binding Buffer (XP2). 5. Incubate at 60°C for 7 minutes or until the gel has completely melted. Vortex or shake the tube every 2-3 minutes.
4. Add 1 volume Binding Buffer (XP2).
5.Incubate at 50-60°C for 7 minutes or until the gel has completely melted. Vortex or shake the tube every 2-3 minutes.
6.Insert a HiBind® DNA Mini Column in a 2 mL Collection Tube.
7.Add no more than 700 μL DNA/agarose solution from Step 5 to the HiBind® DNA Mini Column. Centrifuge at 10,000 x g for 1 minute at room temperature. Discard the ltrate and reuse collection tube.
8.Repeat Steps 7 until all of the sample has been transferred to the column.
9. Add 300 μL Binding Buffer (XP2). Centrifuge at maximum speed (≥13,000 x g) for 1 minute at room temperature. Discard the ltrate and reuse collection tube.
10.Add 700 μL SPW Wash Buffer. Centrifuge at maximum speed for 1 minute at room temperature. Discard the ltrate and reuse collection tube.
11.Centrifuge the empty HiBind® DNA Mini Column for 2 minutes at maximum speed to dry the column matrix. Transfer the HiBind® DNA Mini Column to a clean 1.5 mL microcentrifuge tube.
12.Add 50μL deionized water directly to the center of the column membrane. Centrifuge at maximum speed for 1 minute.
13.Store DNA at -20°C.

The double enzyme digestion system

Put the system into a 37 ° C water bath for half an hour

Ligation

Put the system into a 37°C water bath for half an hour

Chemical Transformation

1. Take competent cells (E.cop DH5α) from -80°C refrigerator and put it on ice. （Set negative control by using chemically competent E.cop cells without plasmids）
2. When the competent cells dissolve (about 10min), add 10 μL DNA pgation product or 2 μL plasmid per tube, Place the mixture on ice for 30 minutes.
3. Heat shock at 42°C for exactly 90 seconds.
4. Put the 1.5 mL tubes back on ice for 3-5 minutes.
5. Add 500 μL LB fluid medium without antibiotics into the 1.5 mL tubes and then cture in the shaker incubator at 37°C for an hour.
6. Extract 100-200 μL bacteria pquid, spread it on LB medium with relevant antibiotic.
7. Place plates upside down and incubate at 37°C overnight.

Colony PCR

using 2×Taq master Mix/2×Hieff PCR Master Mix

Thermocycpng conditions for a Routine PCR:

Plasmid extraction

According to the Plasmid Extraction Mini kit

1. Take 1-5mL bacterial solution into a centrifuge tube, centrifuge at 12,000 rpm for 1 min and remove supernatant.
2. Add 250 μL SolutionⅠ in centrifuge tube, using the pipet or vortex oscillator to suspend the cells.
3. Add 250 μL Solution II in centrifuge tube and gently fpp upside down for 6-8 times to make sure the germ is fl cracked.
4.Add 350 μL Solution III, gently fpp upside down for 6-8 times to mix until white, floccent precipitate appears and centrifuge at 12,000rpm for 10 minutes.
5. Add the supernatant to the adsorption column in step 5, centrifuge at 12,000rpm for l minute, discard the filtrate and reuse collection tube.
6.Add 700 μL Wash solution to the adsorption column, centrifuge at 12,000rpm for l minute, discard the filtrate and reuse collection tube.
7.Add 500 μL Wash solution to the adsorption column, centrifuge at 12,000rpm for l minute, discard the filtrate and reuse collection tube.
8.Centrifuge the empty adsorption column at 12,000rpm for 2 minute to dry the column matrix. (Residual ethanol may impact downstream apppcation)
9.Transfer the adsorption column into a clean 1.5 mL centrifuge tube, add 50 -100μL Elution buffer to the center of the column membrane, let sit at room temperature for 2 minutes and centrifuge at 12,000rpm for l minute, collect the plasmid solution in the centrifuge tube.
10. Store the plasmid at -20 ° C.

LB medium(For 100mL)

Autoclave at 121°C for 20 min.
(1.5g agar shod be added before autoclaving to make sopd LB)

CloneExpress

According to the CloneExpress Mtis One Step Cloning Kit
1).Preparation for the pnearized cloning vectors；
Select appropriate cloning sites, and pnearize the cloning vector.The cloning vectors can be pnearized by restriction digesting with endonuclease or by reverse PCR amppfication.
2).Design of PCR primers of the insertions；
The principle for the design of ClonExpress® MtiS primers is: introduce homologous sequences (15 bp～20 bp)into 5’ end of primers, aiming to making the ends of amppfied insertions and pnearized cloning vector identical to the ends of their neighbours which is required for recombination reaction.
3).PCR amppfication of the insertions；
Insertions can be amppfied by any polymerase (Taq DNA polymerase or other high-fidepty polymerases),but to prevent mutations introduced during PCR, high-fidepty polymerases is highly recommended.
4).Recombination reaction；
Set up the following reaction on ice. Spin briefly to bring the sample to the bottom before reacting.

5).Transformation and plating；
6)Selection of the positive colony .