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JBC, Vol. 252, Issue 8, 2717-2725, Apr, 1977
T. V. Gopalakrishnan and E. B. Thompson
Concanavalin A added to intact cells at 37 degrees caused rapid and
reversible inactivation of a soluble enzyme, tyrosine aminotransferase, in
two lines of rat hepatoma tissue culture cells grown in monolayer culture.
This temperature-dependent process was independent of de novo protein and
RNA synthesis and independent of increased uptake of Ca2+ and Mg2+ or
glucose. The inactivation could be reversed by adding
alpha-methyl-D-mannopyranoside a competing sugar for concanavalin A
binding. Other lectins known to bind to different sugars did not bring
about the inactivation of tyrosine aminotransferase. Addition of
concanavalin A did not result in the inactivation of another soluble
enzyme, lactic dehydrogenase. The maintenance of tyrosine aminotransferase
in an inactive form after the binding of concanavalin A to the cells
required the continued presence of concanavalin A. This effect of
concanavalin A could not be mimicked either by dibutyryl cyclic adenosine
or guanosine monophosphoric acid. Incubation of cell extracts with
concanavalin A did not result in inactivation nor did mixing of extracts
from concanavalin A-treated cells with extracts from untreated cells. On
the basis of these results we conclude that the following are the essential
requirements for concanavalin A to bring about the inactivation of tyrosine
aminotransferase: (a) the binding of native concanavalin A to the cells;
(b) integrity of certain structural elements of the cells.
Effect of concanavalin A on tyrosine aminotransferase in rat hepatoma tissue culture cells. Rapid reversible inactivation of soluble enzyme
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