Affibody molecules are a class of small (∼7 kDa) robust scaffold proteins suitable for radionuclide molecular imaging in vivo. The attachment of a hexahistidine (His(6))-tag to the Affibody molecule allows facile purification by immobilized metal ion affinity chromatography (IMAC) but leads to high accumulation of radioactivity in the liver. Earlier, we have demonstrated that replacement of the His(6)-tag with the negatively charged histidine-glutamate-histidine-glutamate-histidine-glutamate (HEHEHE)-tag permits purification of Affibody molecules by IMAC, enables labeling with [(99m)Tc(CO)(3)](+), and provides low hepatic accumulation of radioactivity. In this study, we compared the biodistribution of cysteine-containing Affibody molecules site-specifically labeled with (111)In, (99m)Tc, and (125)I at the C-terminus, having a His(6)-tag at the N- or C-terminus or a HEHEHE-tag at the N-terminus. We show that the use of a HEHEHE-tag provides appreciable reduction of hepatic radioactivity, especially for radiometal labels. We hope that this information can also be useful for development of other scaffold protein-based imaging agents.
A range of enantiomerically
pure protected side-chain-fluorinated
amino acids has been prepared (13 examples) by treatment of protected
amino acids containing unsaturated side chains with a combination
of Fe(III)/NaBH
4
and Selectfluor. The modification of the
conditions by replacement of Selectfluor with NaN
3
allowed
the preparation of side-chain azido-substituted amino acids (five
examples), which upon catalytic hydrogenation gave the corresponding
amines, isolated as lactams (four examples). Radical hydration of
the unsaturated side chains leading to side-chain-hydroxylated protected
amino acids has also been demonstrated.
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