Fluorine-18 labeling of monoclonal antibodies and fragments with preservation of immunoreactivity |
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Authors: | P K Garg S Garg M R Zalutsky |
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Institution: | Duke University Medical Center, Department of Radiology, Durham, North Carolina 27710. |
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Abstract: | A new method is reported for labeling proteins with the positron-emitting nuclide 18F. Initially, 4-18F]-fluorobenzylamine was prepared in two steps from aqueous 18F]fluoride in high yield. The 18F acylation agent was formed by reaction of this product with disuccinimidyl suberate. Overall yields for the 4-18F]fluorobenzylamine succinimidyl ester (18F]SFBS), decay corrected to the end of cyclotron bombardment, were about 30% in a synthesis time of 60 min. After a 15-min reaction, 30-45% (decay corrected) of the 18F]SFBS could be coupled to intact antibodies and their F(ab')2 and Fab fragments. Coupling yields were dependent on protein concentration but not reaction time. HPLC purification of 18F]SFBS was necessary to obtain optimal coupling efficiency and immunoreactivity. The immunoreactivities of 18F-labeled F(ab')2 and Fab fragments of an antimyosin antibody were 89 +/- 5% and 75 +/- 9%, respectively. Biodistribution studies in normal mice demonstrated similar in vivo behavior of 18F-labeled antibody fragments and those labeled with 125I by using N-succinimidyl 3-125I]iodobenzoate. These results indicate that this method may be useful for labeling monoclonal antibodies and other proteins and peptides with 18F. |
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