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A novel anti-aldolase C antibody specifically interacts with residues 85-102 of the protein.

S. Langellotti
•
ROMANO, MAURIZIO
•
C. Guarnaccia
altro
F. Salvatore
2014
  • journal article

Periodico
MABS
Abstract
Aldolase C is a brain-specific glycolytic isozyme whose complete repertoire of functions are obscure. This lack of knowledge can be addressed using molecular tools that discriminate the protein from the homologous, ubiquitous paralog aldolase A. The anti-aldolase C antibodies currently available are polyclonal and not highly specific. We obtained the novel monoclonal antibody 9F against human aldolase C, characterized its isoform specificity and tested its performance. First, we investigated the specificity of 9F for aldolase C. Then, using bioinformatic tools coupled to molecular cloning and chemical synthesis approaches, we produced truncated human aldolase C fragments, and assessed 9F binding to these fragments by western blot and ELISA assays. This strategy revealed that residues 85-102 harbor the epitope-containing region recognized by 9F. The efficiency of 9F was demonstrated also for immunoprecipitation assays. Finally, surface plasmon resonance revealed that the protein has a high affinity toward the epitope-containing peptide. Taken together, our findings show that epitope recognition is sequence-driven and is independent of the three-dimensional structure. In conclusion, given its specific molecular interaction, 9F is a novel and powerful tool to investigate aldolase C's functions in the brain.
DOI
10.4161/mabs.28191
WOS
WOS:000335384800011
Archivio
http://hdl.handle.net/11368/2784330
info:eu-repo/semantics/altIdentifier/scopus/2-s2.0-84899744885
http://dx.doi.org/10.4161/mabs.28191
Diritti
metadata only access
Soggetti
  • Aldolase C

  • brain

  • monoclonal antibody

  • Epitope mapping

  • Western blotting

  • ELISA assay

Web of Science© citazioni
6
Data di acquisizione
Mar 23, 2024
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