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Department of Medicine, Medical University of South Carolina and the Medical and Research Services, Ralph H. Johnson Veterans Affairs Medical Center, Charleston, South Carolina 29425
Early passage
mesangial cells, like many other nonimmortalized cultured cells, can be
difficult to transfect. We devised a simple method to improve the
efficiency of transient protein expression under the transcriptional
control of promoters in conventional plasmid vectors in rat mesangial
cells. We used a vector encoding modified green fluorescent protein
(GFP) and sterile fluorescence-activated cell sorting (FACS) to select
a population consisting of >90% GFP-expressing cells from passaged
nonimmortalized cultures transfected at much lower efficiency. Only
10% transfection efficiency was noted with a
-galactosidase
expression vector alone, but cotransfection with GFP followed by FACS
and replating of GFP+ cells
yielded greater than fivefold enrichment of cells with detectable
-galactosidase activity. To demonstrate the expression of a properly
oriented and processed membrane protein, we cotransfected GFP with a
natriuretic peptide clearance receptor (NPR-C) expression vector.
Plasmid-dependent cell surface NPR-C density was enhanced by 89% after
FACS, though expression remained lower in selected mesangial cells than
in the CHO cell line transfected with the same vector. We conclude that
cotransfection of rat mesangial cells with GFP, followed by FACS,
results in improvement in transient transfection efficiencies to levels
that should suffice for many applications.
automated cell sorting; adenovirus; lipofection; liposome
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