JOURNAL ARTICLE

Transfection Using DEAE‐Dextran

Tod Gulick

Year: 1997 Journal:   Current Protocols in Neuroscience Vol: 1 (1)Pages: Appendix 1D-Appendix 1D   Publisher: Wiley

Abstract

Abstract Transfection of cultured mammalian cells using diethylaminoethyl (DEAE)‐dextran/DNA can be an attractive alternative to other transfection methods in many circumstances. The major advantages of the technique are its relative simplicity and speed, limited expense, and remarkably reproducible interexperimental and intraexperimental transfection efficiency. Disadvantages include inhibition of cell growth and induction of heterogeneous morphological changes in cells. Furthermore, the concentration of serum in the culture medium must be transiently reduced during the transfection. In general, DEAE‐dextran DNA transfection is ideal for transient transfections with promoter/reporter plasmids in analyses of promoter and enhancer functions, and is suitable for overexpression of recombinant protein in transient transfections or for generation of stable cell lines using vectors designed to exist in the cell as episomes. This unit presents a general description of DEAE‐dextran transfection, as well as two more specific protocols for typical experimental applications. The basic protocol is suitable for transfection of anchorage‐dependent (attached) cells. For cells that grow in suspension, electroporation or lipofection is usually preferred, although DEAE‐dextran‐mediated transfection can be used.

Keywords:
Dextran Transfection Chemistry Computer science Cell biology Biology Biochemistry Gene

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Citation History

Topics

RNA Interference and Gene Delivery
Life Sciences →  Biochemistry, Genetics and Molecular Biology →  Molecular Biology
Virus-based gene therapy research
Life Sciences →  Biochemistry, Genetics and Molecular Biology →  Genetics
Advanced biosensing and bioanalysis techniques
Life Sciences →  Biochemistry, Genetics and Molecular Biology →  Molecular Biology

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