A simplified workflow for monoclonal antibody sequencing.
Lena MeyerTomás LópezRafaela EspinosaCarlos F AriasChristopher VollmersRebecca M DuBoisPublished in: PloS one (2019)
The diversity of antibody variable regions makes cDNA sequencing challenging, and conventional monoclonal antibody cDNA amplification requires the use of degenerate primers. Here, we describe a simplified workflow for amplification of IgG antibody variable regions from hybridoma RNA by a specialized RT-PCR followed by Sanger sequencing. We perform three separate reactions for each hybridoma: one each for kappa, lambda, and heavy chain transcripts. We prime reverse transcription with a primer specific to the respective constant region and use a template-switch oligonucleotide, which creates a custom sequence at the 5' end of the antibody cDNA. This template-switching circumvents the issue of low sequence homology and the need for degenerate primers. Instead, subsequent PCR amplification of the antibody cDNA molecules requires only two primers: one primer specific for the template-switch oligonucleotide sequence and a nested primer to the respective constant region. We successfully sequenced the variable regions of five mouse monoclonal IgG antibodies using this method, which enabled us to design chimeric mouse/human antibody expression plasmids for recombinant antibody production in mammalian cell culture expression systems. All five recombinant antibodies bind their respective antigens with high affinity, confirming that the amino acid sequences determined by our method are correct and demonstrating the high success rate of our method. Furthermore, we also designed RT-PCR primers and amplified the variable regions from RNA of cells transfected with chimeric mouse/human antibody expression plasmids, showing that our approach is also applicable to IgG antibodies of human origin. Our monoclonal antibody sequencing method is highly accurate, user-friendly, and very cost-effective.
Keyphrases
- monoclonal antibody
- endothelial cells
- poor prognosis
- amino acid
- single cell
- nucleic acid
- escherichia coli
- stem cells
- cell therapy
- long non coding rna
- immune response
- induced pluripotent stem cells
- high resolution
- transcription factor
- palliative care
- nuclear factor
- binding protein
- pluripotent stem cells
- toll like receptor
- oxidative stress
- signaling pathway
- label free
- inflammatory response
- multidrug resistant