| Literature DB >> 31882320 |
Trudy Straetemans1, Anke Janssen2, Koen Jansen2, Ruud Doorn2, Tineke Aarts2, Anna D D van Muyden2, Marieke Simonis3, Judith Bergboer3, Moniek de Witte2, Zsolt Sebestyen2, Jurgen Kuball4.
Abstract
Despite extensive usage of gene therapy medicinal products (GTMPs) in clinical studies and recent approval of chimeric antigen receptor (CAR) T cell therapy, little information has been made available on the precise molecular characterization and possible variations in terms of insert integrity and vector copy numbers of different GTMPs during the complete production chain. Within this context, we characterize αβT cells engineered to express a defined γδT cell engineered to express a defined γδT receptor (TEG) currently used in a first-in-human clinical study (NTR6541). Utilizing targeted locus amplification in combination with next generation sequencing for the vector producer clone and TEG001 products, we report on five single-nucleotide variants and nine intact vector copies integrated in the producer clone. The vector copy number in TEG001 cells was on average a factor 0.72 (SD 0.11) below that of the producer cell clone. All nucleotide variants were transferred to TEG001 without having an effect on cellular proliferation during extensive in vitro culture. Based on an environmental risk assessment of the five nucleotide variants present in the non-coding viral region of the TEG001 insert, there was no altered environmental impact of TEG001 cells. We conclude that TEG001 cells do not have an increased risk for malignant transformation in vivo.Entities:
Keywords: GTMP; TEG001; TLA; engineered T cells; gene therapy medicinal product; targeted locus amplification; vector copy number; γδT cells
Year: 2019 PMID: 31882320 PMCID: PMC7001055 DOI: 10.1016/j.ymthe.2019.11.030
Source DB: PubMed Journal: Mol Ther ISSN: 1525-0016 Impact factor: 11.454