ull is considered to be useful for the study on the manner of the hydrogen bonding of polypeptides and proteins. (21) Harbison, G. S.; Jelinski, L. W.; Stark, R. E.; Torchia, D. A.; Herzfeld, J.; Griffin, R. G. J. Magn. Reson. 1984, 60, 79-82.
Three kinds of 2H-labeled Bombyx mori silk
fibroin samples (with [2,2-2H2]Gly,
[3,3,3-2H3]Ala, or [2,3,5,6-2H4]Tyr) were obtained
by oral administration of either the labeled amino acid or
2H2O to
5th instar larvae. The administration of
2H2O alone yielded a high degree of selective
deuteration at the
alanine methyl group, since the incorporation of
2H2O occurs between fumarate and malate in
the
tricarboxylic acid (TCA) cycle of the silk fibroin synthetic pathway.
Uniaxially oriented silk fibers were
prepared as samples for 2H-NMR spectroscopy. An
analysis of the quadrupole echo line shape was carried
out in order to determine the angle of the deuterium-labeled group
relative to the fiber axis, i.e., of the
Cα−2H bond vectors in glycine and of
Cα−Cβ2H3 in alanine. With the fiber
axis aligned parallel to the
magnetic field, quadrupole splittings were obtained as 117.8 and 39.8
kHz for [2,2-2H2]Gly- and
[3,3,3-2H3]Ala-labeled silk, respectively.
These values are identical with those obtained from the
2H-NMR powder
patterns of the unaligned samples, within experimental error. From
the angular dependence of the
quadrupole splittings, it was thus calculated that the
Cα−2H bonds of glycine as well as the
Cα−Cβ2H3
bond of alanine make an angle of approximately 90° relative to the
fiber axis. These steric constraints
were then used to evaluate the torsion angles, φ and ψ,
for the glycine and alanine residues within the
protein backbone. These data, determined independently by
solid-state 2H NMR, thus verified and
narrowed down the allowed region in the Ramachandran (φ,
ψ) map obtained from previous solid-state
13C- and 15N-NMR studies.
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