Journal of Translational Medicine (Jul 2007)

Molecular purging of multiple myeloma cells by <it>ex-vivo </it>culture and retroviral transduction of mobilized-blood CD34<sup>+ </sup>cells

  • Corneo Gianmarco,
  • Pogliani Enrico,
  • Monari Marta,
  • Vai Sergio,
  • Voena Claudia,
  • Dando Jonathan,
  • Ficara Francesca,
  • Cergnul Massimiliano,
  • Birolo Roberto,
  • Scaramuzza Samantha,
  • Deola Sara,
  • Peccatori Jacopo,
  • Selleri Silvia,
  • Bordignon Claudio,
  • Roncarolo Maria,
  • Aiuti Alessandro,
  • Bregni Marco

DOI
https://doi.org/10.1186/1479-5876-5-35
Journal volume & issue
Vol. 5, no. 1
p. 35

Abstract

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Abstract Background Tumor cell contamination of the apheresis in multiple myeloma is likely to affect disease-free and overall survival after autografting. Objective To purge myeloma aphereses from tumor contaminants with a novel culture-based purging method. Methods We cultured myeloma-positive CD34+ PB samples in conditions that retained multipotency of hematopoietic stem cells, but were unfavourable to survival of plasma cells. Moreover, we exploited the resistance of myeloma plasma cells to retroviral transduction by targeting the hematopoietic CD34+ cell population with a retroviral vector carrying a selectable marker (the truncated form of the human receptor for nerve growth factor, ΔNGFR). We performed therefore a further myeloma purging step by selecting the transduced cells at the end of the culture. Results Overall recovery of CD34+ cells after culture was 128.5%; ΔNGFR transduction rate was 28.8% for CD34+ cells and 0% for CD138-selected primary myeloma cells, respectively. Recovery of CD34+ cells after ΔNGFR selection was 22.3%. By patient-specific Ig-gene rearrangements, we assessed a decrease of 0.7–1.4 logs in tumor load after the CD34+ cell selection, and up to 2.3 logs after culture and ΔNGFR selection. Conclusion We conclude that ex-vivo culture and retroviral-mediated transduction of myeloma leukaphereses provide an efficient tumor cell purging.