Structural Biochemistry/DNA recombinant techniques/Electroporation

< Structural Biochemistry < DNA recombinant techniques

Overview

Electroporation can be used to insert genes into eukaryotic cells such as plants cells and animal cells, as well as prokaryotic cells such as bacterial cells. In electroporation, cereal monocots and dicots can be introduced to foreign DNA by applying intense electric fields.

Procedure

Lets take a plant cell as an example. First, a plant cell will consist of a cell wall and a plasma membrane. Cellulose is used to digest the cell wall, creating a plant cell that is has an exposed membrane. This is known as a protoplast. Second, foreign DNA is added into the cell. High electric fields are used to create a transiently permeable membrane so that large molecules will be able to pass through the membrane. This is caused by transient electric pulses. Thirdly, the cell wall is able to regrow back. In the end, the plant cell is now a viable plant cell with an insert of foreign DNA.

Considerations for Optimization[1]

When in vitro electroporation is performed, there are several factors that must be taken into account.

Importance

Electroporation is usually used in molecular biology to introduce a substance into a cell. This can be done with a molecular probe loading the substance into the cell, by a piece of coding DNA, or by a drug that is able to change the functions of a cell. Electroporation is highly efficient when trying to introduce foreign genes into tissue culture cells. An example is mammalian cells. This process is used in the production of knockout mice. Electroporation is beneficial because it can be used to treat tumors, as well as cell-based therapy and gene therapy. This is known as transfection, the process that is used to introduce foreign DNA into eukaryotic cells.

  1. Gehl, J. "Electroporation: theory and methods, perspectives for drug delivery, gene therapy, and research." Acta Physion Scand 177 (2002): 437-447.
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