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J. Biol. Chem., Vol. 255, Issue 6, 2454-2456, 03, 1980
T Yubisui and M Takeshita
NADH-cytochrome b5 reductase of normal human erythrocytes was purified by
procedures including affinity chromatography on Blue-Sepharose to an
electrophoretically homogeneous protein. The purified enzyme was judged to
be a typical flavoprotein based on its absorption spectrum (absorption
maxima, 272, 390, and 462 nm; shoulders, 373 and 488 nm) and flavin content
(1 mol of FAD/mol of enzyme). The minimum molecular weight calculated from
the flavin content was 32,300. The purified enzyme showed a distinct
negative circular dichroic spectrum at 280 nm and also at 460 to 480 nm.
With the best preparations, the molar ellipticities at 280 and 460 nm were
well correlated with the enzyme activity and flavin content in the enzyme.
A partial loss of flavin from the enzyme led to a concomitant loss of
enzyme activity and decrease in the molar ellipticities at 460 and 280 nm.
Flavin analogues such as acrinol and proflavine (0.1 mM) strongly inhibited
the enzyme activity, and atebrin (0.1 mM) also showed partial inhibition.
Complete inhibition was observed with 1 mM of any these reagents. These
results apparently indicate that FAD in the enzyme functions as a
prosthetic group, and that circular dichroic spectroscopy is a good measure
of the bound form of flavin in the enzyme.
Characterization of the purified NADH-cytochrome b5 reductase of human erythrocytes as a FAD-containing enzyme
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