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J. Biol. Chem., Vol. 261, Issue 20, 9155-9160, 07, 1986
Structural basis of human erythrocyte glucose transporter function in reconstituted system. Hydrogen exchange
EK Jung, JJ Chin and CY Jung
Hydrogen exchange kinetic behavior of human erythrocyte glucose transporter
protein in vesicles was studied in the absence and in the presence of
D-glucose or a well known inhibitor, cytochalasin B. This is to detect a
proposed channel of water penetrating into the protein through which the
sugar molecule passes and to monitor any conformational changes induced by
the substrate or inhibitor. Analyses of the kinetic data revealed several
classes of hydrogens which exchange with readily distinguishable rates. Of
660 hydrogens detected per transporter, approximately 30% exchanged with
rates generally characterized as those of free amide hydrogens indicating
they are interfaced to solvent water. Since the transporter is known to be
embedded deep in the hydrophobic area of the membrane with minimum exposure
to the outside of the membrane lipid bilayer, a significant portion of
these free amide hydrogens must be at the purported channel rather than
outside of the membrane. D-Glucose and cytochalasin B affected the exchange
kinetics of these presumably channel-associated free amide hydrogens rather
differently. D-Glucose reduced the apparent rate constants, but not the
total number. Cytochalasin B on the other hand reduced the total number to
one-half without significantly changing the apparent rate constants. The
remaining 70% of the labeled hydrogens exchanged with much slower rates
which vary 10-10,000-fold, indicating that they are internally structured
peptide amide and side chain hydrogens. Both D-glucose and cytochalasin B
further reduced the rates of these hydrogens, indicating a global
stabilization of the protein structure.

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Copyright © 1986 by the American Society for Biochemistry and Molecular Biology.
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