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Vol. 301, Issue 3, 812-819, June 2002
Department of Pharmacobio-dynamics, Faculty of Pharmaceutical
Sciences, Kanazawa University, Takara-machi, Kanazawa, Japan (H.T.,
Y.S., I.T., A.T.); and Core Research for Evolutional Science and
Technology, Japan Science and Technology Corporation, Moto-machi,
Kawaguchi, Japan (Y.S., I.T., A.T.)
To explore the feasibility of drug delivery to the liver by
the use of adenovirus-mediated human oligopeptide transporter (hPEPT1) gene transfer, we examined the accumulation of
L-[3H]carnosine in the hepatoma cell line
(HepG2 and WIFB9) and mouse liver. We constructed a recombinant
adenovirus encoding hPEPT1-enhanced yellow fluorescent protein (EYFP)
fusion gene (AdhPEPT1-EYFP). In vitro uptake of
L-[3H]carnosine was determined in HepG2 and
WIFB9 cells transduced with AdhPEPT1-EYFP. In vivo, the accumulation of
L-[3H]carnosine in mouse liver was evaluated
after transduction of AdhPEPT1-EYFP. At pH 6.0, the uptake of
L-[3H]carnosine by HepG2 and WIFB9 cells
transduced with AdhPEPT1-EYFP was increased 15- and 2-fold,
respectively, compared with the cells without transduction. At pH 7.4, uptake of L-[3H]carnosine in AdhPEPT1-EYFP
transduced HepG2 cells was 3 times greater than that of nontransduced
cells. In the presence of carnosine or glycylsarcosine as an inhibitor
at 20 mM, the uptake of L-[3H]carnosine was
reduced to a level comparable to that of nontransduced cells. At 30 min
after intravenous administration of
L-[3H]carnosine to mice transduced with
AdhPEPT1-EYFP at 1 × 1010 plaque-forming
units/mouse, the tissue-to-plasma concentration ratio
(Kp) of
L-[3H]carnosine in the liver was
significantly increased to 7 times that of nontransduced mice. In
contrast, the Kp value of
[14C]inulin, a marker for extracellular fluid space,
remained unchanged after adenoviral transduction suggesting minimal
pathological damage of tissues. hPEPT1-EYFP was localized at both the
basolateral and apical membranes in HepG2 cells, WIFB9 cells, and mouse
liver. In conclusion, our results suggest that delivery of oligopeptide to the liver by adenovirus-mediated heterologous expression of hPEPT1
in vivo is feasible.
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