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Development of a high-throughput RT-PCR based viral infectivity assay for monitoring the stability of a replicating recombinant Lymphocytic Choriomeningitis viral vector

J Virol Methods. 2021-12; 
Vineet Gupta, Lorena R Antunez, Soraia Saleh-Birdjandi, Ozan S Kumru, Richard Pospisil, Anders Lilja, Gerhard Fuhrmann, Lee Smith, David B Volkin, Sangeeta B Joshi
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Proteins, Expression, Isolation and Analysis … Briefly, the coding sequence of the HPV16 vaccine antigen, fusion protein of E7 and E6 (Genbank accession # K02718) with five mutations was synthesized by Genscript and inserted?… Get A Quote

摘要

Traditional virus infectivity titration methods for lymphocytic choriomeningitis virus (LCMV) are laborious, time-consuming, and low-throughput (e.g., focus forming unit (FFA) assay). In this report, we developed a high-throughput reverse transcription quantitative PCR (RT-qPCR)-based virus infectivity assay for relative quantitation of a live, recombinant replicating LCMV -based viral vector (TT1). This in vitro infectivity assay demonstrated a 4-log linear range for TT1 titer quantitation. A high positive Pearson correlation coefficient value (≥ 0.80) was obtained between the RT-qPCR vs. the "gold-standard" FFU assay when comparing the stability profiles of stressed TT1 vector samples. In addition to the RT... More

關鍵詞

Focus forming unit (FFU), Formulation, Replicating recombinant lymphocytic choriomeningitis virus (TT1), Reverse transcription quantitative PCR (RT-qPCR), Stability, Viral vector
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