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Merck

Retroviral transduction of murine primary T lymphocytes.

Methods in molecular biology (Clifton, N.J.) (2008-12-27)
James Lee, Michel Sadelain, Renier Brentjens
ABSTRACT

In comparison to human T cells, efficient retroviral gene transfer and subsequent expansion of murine primary T cells is more difficult to achieve. Herein, we describe an optimized gene transfer protocol utilizing an ecotropic viral vector to transduce primary murine T cells activated with magnetic beads coated with agonistic anti-CD3 and CD28 antibodies. Activated T cells are subsequently centrifuged (spinoculated) on RetroNectin-coated tissue culture plates in the context of retroviral supernatant. Variables found to be critical to high gene transfer and subsequent efficient T cell expansion included CD3/CD28 magnetic bead to cell ratio, time from T cell activation to initial spinoculation, frequency of T cell spin-oculation, interleukin-2 concentration in the medium, and the initial purity of the T cell preparation.

MATERIALI
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Roche
Interleukin-2, mouse (mIL-2), recombinant (E. coli)