Electroporation of Cas12a RNP (ribonucleoprotein) into adherent cells using the Neon® Electroporation

 

Overview:

EnGen Lba Cas12a (Cpf1) Nuclease (NEB #M0653) may be used in vivo to create targeted genome modifications. There are several ways in which to introduce Cas12a-guide RNA complexes into cells. Here we present a method for the introduction of Cas12a RNP’s into HEK293 FT cells using the Thermo Fisher® Neon Electroporation System. This method uses 100 pmoles of EnGen Lba Cas12a and 1000 pmol of guide RNA per transfection in a 24-well culture plate.

Required Materials:

Cell Culture and Transfection

  •                 HEK293 cells (or other cell line) at 70-90% confluency in a T-75 flask

  •                 EnGen® Lba Cas12a (Cpf1) (NEB #M0653)[WJ1]

  •                 gRNA containing the targeting sequence in the region of interest

  •                 ThermoFisher Neon Transfection System 10 µl Kit (MPK1025)

  •                 Sterile 1X PBS without Ca2+and Mg2+

  •                 DMEM with Glutamax (or appropriate growth medium) with 10% FBS

  •                 24-well culture plate

  •  

    DNA Extraction and Genome Editing Analysis

  •                 EnGen Mutation Detection Kit (NEB #E3321)

  •                 Epicentre QuickExtract™ DNA Extraction Solution (Epicentre #QE09050)

     

    Before You Start:

  • We strongly recommend wearing gloves and using nuclease-free tubes and reagents to avoid RNase contamination. Further recommendations for avoiding ribonuclease contamination can be found here. Please hyperlink underlined text to  https://www.neb.com/tools-and-resources/usage-guidelines/avoiding-ribonuclease-contamination

  • Please refer to the Neon Transfection System manual for proper usage of the equipment.

     

  • The Neon 10 µl Transfection System draws 10 µl of cells and transfection material into an electroporation pipette tip. This tip may be used twice for two sequential electroporations. Therefore, the volumes in this protocol are for duplicate reactions set up in the same tube, with an overage of 5 µl. However, volumes can be adjusted according to the user’s needs.

     

     

    Protocol:

    Electroporation

  1. Seed the cells so that they will be around 70-90% confluent on the day of transfection.

  2. Set up the RNP formation reaction as follows below. The volumes below will allow for two (2) electroporations (with addition of cells) of 10 µl, with an overage of 5.0 µl. Volumes can be adjusted to allow for more overage if necessary, or to perform single electroporation reactions:

     

COMPONENT [MD2]

AMOUNT

Resuspension Buffer R

7.0 µl

EnGen Lba Cas12a (Cpf1) (100 µM)

2.5 µl

gRNA (500 µM)

5.0 µl

Total Reaction Volume

14.5 µl

 

 

  1. Gently mix the Resuspension Buffer R, EnGen Lba Cas12a, and gRNA [MD3]and incubate at room temperature for 20 minutes.

     

  2. During the incubation, trypsinize the cells, washing once to remove any traces of trypsin. Resuspend the cells in 5-10 ml of media. Dilute 20 μl of the cells with 20 μl of trypan blue. Determine the cell number and viability using a hemacytometer.

 

  1. Calculate the number of cells you will need for the entire experiment (1-2 x 105 cells per duplicate transfection) and move those to a sterile microfuge tube. Pellet for 5 min at 500 x g. Wash the cells once with 1X PBS and repeat the centrifugation.

 

  1. Calculate the volume of Resuspension Buffer R you will need to resuspend the cells (10.5 µl for duplicate transfections). Resuspend the cells in your calculated volume.

     

  2. Prepare a 24-well plate by adding 500 µl growth medium to the appropriate number of wells.

     

  3. Add 10.5 µl of cells to each 14.5 µl RNP reaction.

 

 

  1. Aspirate 10 µl of the RNP/cells mix into a 10 µl Neon tip. Electroporate the cells under the following conditions: 1700V, 20 ms, 1 pulse.

     

  2. Immediately transfer the cells to the prepared 24-well plate. Repeat with the next 10 µl and the same electroporation tip if desired.

     

  3. Incubate the cells in a humidified 37°C, 5% CO2 incubator for 48-72 hours.

     

    Harvest DNA for on-target editing analysis

  1. Gently aspirate the media from the cells and wash twice with 100 µl 1X PBS. 

     

  2. Add 50 µl of Epicentre QuickExtract DNA Extraction Solution and shake/vortex for 5 minutes. Transfer the solution to a PCR plate or tubes and place in a thermocycler, running the following program:

     

  • 65°C for 15 min

     

  • 95°C for 15 min

     

  • Hold at 4°C

     

  1. DNA may be used undiluted or diluted. Amplification of the target region may need optimization.

  2. For genome editing analysis, follow the protocol detailed in the EnGen Mutation Detection Kit (NEB #E3321) manual


 [WJ1]Links needs to be updated for M0653

 [MD2]Brian, please set up in your normal table styles format

 [MD3]This is a little confusing to me. It looks like the cells are added at this step because they are included in the table. Perhaps we should remove them and adjust total reaction volume?

 

JW: removed volume of cells from table.