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1 Department of Internal
Medicine,
The Cre/loxP and Flp/FRT systems mediate site-specific DNA
recombination and are being increasingly utilized to study gene function in vivo. These systems allow targeted gene disruption in a
single cell type in vivo, thereby permitting study of the physiological
and pathophysiological impact of a given gene product derived from a
particular cell type. In the kidney, the Cre/loxP system has been
employed to achieve gene deletion selectively within principal cells of
the collecting duct. Disruption of target genes in the collecting duct,
such as endothelin-1 or polycystic kidney disease-1
(PKD1), could lead to important insights into the
biological roles of these gene products. With selection of the
appropriate renal cell-specific promoters, these recombination systems
could be used to target gene disruption to virtually any renal cell
type. Although transgenic studies utilizing these recombination systems
are promising, they are in their relative infancy and can be time
consuming and expensive and yield unanticipated results. It is anticipated that continued experience with these systems will
produce an important tool for analyzing gene function in renal health
and disease.
Cre recombinase; loxP; aquaporin-2
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