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(Received for publication, May 9, 1997, and in revised form, July 28, 1997)
,§
From the Departments of Cationic liposomes are potentially important gene
transfer vehicles, although their application has been limited by
relatively low efficiency of transgene expression. Single cell
quantitative methods, such as those used in this study, should permit a
more detailed understanding of the relationships between delivered plasmid and transgene expression. Intracellular plasmid delivery and
transgene expression were measured simultaneously using photoconjugated ethidium monoazide as an intracellular plasmid delivery marker and
green fluorescent protein (GFP(S65T)) as a transgene expression marker.
Quantitative flow cytometry was used to estimate plasmid copy number
and GFP(S65T) molecules in single cells. The plasmid was delivered to
HeLa cells with a cationic liposome vehicle containing 1,2-dioleoyloxy-3-trimethylammonium-propane and
dioleoylphosphatidylethanolamine (1:1 mol/mol). Treatment was carried
out continuously for 24 h. Flow cytometry measurements on 20,000 cells were performed during treatment and for 48 h post-treatment.
On a single cell basis, transgene expression efficiency and average
GFP(S65T) expression level increased with intracellular plasmid copy
number. After 3-h exposure to the liposomal vector, more than 95% of
the cells were positive for plasmid entry, but none had detectable
transgene expression. Maximum transgene expression was achieved at
24 h and remained unchanged at the 72-h measurement. At 24 h,
the average positive cell contained 1.6 × 105
plasmid copies and 2.3 × 106 GFP(S65T) molecules.
Importantly, the measurement strategies revealed that transgene
expression varied widely within the entire cell population. Although
only 30% of all cells expressed transgene, the subpopulation of cells
that rapidly incorporated the vector demonstrated 100% efficiency in
transgene expression. This study identifies parameters that modulate
highly efficient transgene expression from plasmid delivery by cationic
liposomes.
Chemical and
§ Biomedical Engineering, Vanderbilt University,
Nashville, Tennessee 37235
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