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J. Biol. Chem., Vol. 262, Issue 26, 12550-12556, Sep, 1987
P Ghosh and S Chatterjee
We have previously shown that cultured human proximal tubular cells (PT)
incubated with gentamicin contain numerous "myeloid bodies." This
morphological change was accompanied by the storage of phosphatidylcholine
and sphingomyelin. In order to delineate the biochemical mechanisms
responsible for the accumulation of sphingomyelin in cells incubated with
gentamicin, we pursued detailed studies on the activity of
sphingomyelinase. Characterization studies on sphingomyelinase revealed
that this enzyme has a bimodal pH optima in PT cells. Optimum activity was
observed at pH 5.6 (designated as acid sphingomyelinase, A-SMase) and at pH
7.4 (designated as neutral sphingomyelinase, N-SMase). The activity of both
the enzymes increased proportionately in control cells as a function of
days of incubation. The activity of A-SMase was 16% lower in cells
incubated with gentamicin as compared to control. The most striking
observation was a gradual decline in the activity of N-SMase in cells
incubated with gentamicin. Thus, following 21 days of incubation of cells
with 0.3 mM gentamicin, the N-SMase was 2.7-fold lower than control cells.
Mg2+ stimulated and Triton X-100 inhibited the activity of N-SMase. Whereas
Mg2+ had no effects, Triton X-100 stimulated the activity of the A- SMase
in PT cells. Moreover, A-SMase was relatively more heat-resistant than the
N-SMase. The Km values for sphingomyelin using A-SMase in control cells and
cells incubated with gentamicin were 0.07 X and 0.016 X 10(-7) M,
respectively, whereas the Km values for sphingomyelin using N-SMase in
control cells and cells incubated with gentamicin were 1.8 X and 1.5 X
10(-7) M, respectively. These findings suggest that gentamicin exerts a
competitive inhibition of the A-SMase in PT cells. In contrast, gentamicin
exerts a noncompetitive inhibition of the N- SMase in PT cells. Subcellular
fractionation studies revealed that A- SMase was exclusively localized in
the "lysosome-rich" fraction, whereas most, if not all, the N-SMase was
localized in the microsomal fraction and "plasma-membrane"-rich fraction in
cultured PT cells. Cells incubated with gentamicin for 21 days contained
25% lower activity of A-SMase associated with the lysosomal fraction as
compared to control. In contrast, N-SMase activity in the microsomal and
plasma membrane fraction was one-half as compared to control. We conclude
that gentamicin-mediated decrease in sphingomyelinase activity may be
responsible for the storage of sphingomyelin in cultured human PT
cells.(ABSTRACT TRUNCATED AT 400 WORDS)
Effects of gentamicin on sphingomyelinase activity in cultured human renal proximal tubular cells
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