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A Novel High-Throughput Technique for Identifying Monoclonal Antibodies Capable of Death Receptor Induced Apoptosis. | LitMetric

AI Article Synopsis

  • The study focuses on death receptor family-induced apoptosis, specifically targeting DR4 and DR5 with therapeutic antibodies, which have shown success in clinical trials.
  • The search for effective antibodies targeting the Fas receptor has been challenging due to the differences in behavior of antibodies in lab settings compared to living organisms.
  • A new high-throughput screening method has been developed to identify potential therapeutic antibodies that can effectively induce apoptosis by artificially cross-linking those bound to the Fas receptor.

Article Abstract

The study of death receptor family induced apoptosis has gained momentum in recent years with the knowledge that therapeutic antibodies targeting DR4 and DR5 (death receptor's 4 and 5) have proved efficacious in multiple clinical trials. The therapeutic rationale is based on targeting and amplifying a tumour tissues normal cell death programme (apoptosis). While advances in the targeting of DR4 and DR5 have been successful the search for an agonistic antibody to another family member, the Fas receptor, has proven more elusive. This is partly due to the differing in vitro and in vivo characteristics of individual antibodies. In order to induce Fas targeted cell death an antibody must be capable of binding to and trimerising the receptor. It has been shown that antibodies capable of performing this function in vivo, with the assistance of tumour associated cells, do not always induce apoptosis in vitro. As a result the use of current methodologies to detect functional antibodies in vitro may have dismissed potential therapeutic candidates ('false negative'). Here we report a novel high throughput screening technique which artificially cross-links antibodies bound to the Fas receptor. By combining this process with Annexin-V and Prodidium Iodide (PI) staining we can select for antibodies which have the potential to induce apoptosis in vivo.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC4474333PMC
http://dx.doi.org/10.4137/jcd.s3660DOI Listing

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