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Antiferritin VL homodimer binds human spleen ferritin with high specificity




TekijätNymalm Y, Kravchuk Z, Salminen T, Chumanevich AA, Dubnovitsky AP, Kankare J, Pentikainen O, Lehtonen J, Arosio P, Martsev S, Johnson MS

KustantajaACADEMIC PRESS INC ELSEVIER SCIENCE

Julkaisuvuosi2002

JournalJournal of Structural Biology

Tietokannassa oleva lehden nimiJOURNAL OF STRUCTURAL BIOLOGY

Lehden akronyymiJ STRUCT BIOL

Artikkelin numeroPII S1047-8477(02)00015-1

Vuosikerta138

Numero3

Aloitussivu171

Lopetussivu186

Sivujen määrä16

ISSN1047-8477

DOIhttps://doi.org/10.1016/S1047-8477(02)00015-1


Tiivistelmä
The antiferritin variable light domain (VL) dimer binds human spleen ferritin (similar to85% L subunits) but with similar to50-fold lower affinity, K-a = 4 x 10(7)M(-1), than the parent F11 antibody (K-a = 2.1 x 10(9)M(-1)). The VL dimer does not recognize either rL (100% L subunits) or rH (100% H subunits) human ferritin, whereas the parent antibody recognizes rL-ferritin. To help explain the differences in ferritin binding affinities and specificities, the crystal structure of the VL domain (2.8 Angstrom resolution) was determined by molecular replacement and models of the antiferritin VL-VH dimer were made on the basis of antilysozyme antibody D1.3. The domain interface is smaller in the VL dimer but a larger number of interdomain hydrogen bonds may prevent rearrangement on antigen binding. The antigen binding surface of the VL dimer is flatter, lacking a negatively charged pocket found in the VL-VH models, contributed by the CDR3 loop of the VH domain. Loop CDR2 (VL dimer) is located away from the antigen binding site, while the corresponding loop of the VH domain would be located within the antigen binding site. Together these differences lead to 50-fold lower binding affinity in the VL dimer and to more restricted specificity than is seen for the parent antibody. (C) 2002 Elsevier Science (USA). All rights reserved.



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