Abstract
Early work from a number of laboratories has demonstrated the low frequency with which peripheral human B cells secreting specific monoclonal antibodies can be rescued by cell fusion (Olsson et al., 1983; Kozbor and Roder, 1983b, 1984). Use of spleen and lymph node tissue only marginally improved these results. The development of new human fusion partners (Larrick et al.,1983; Glassy et al., 1983; Kozbor and Roder, 1983; Chiorazzi et al., 1982; Abrams et al., 1983), mouse—human heteromyeloma cell lines (Teng et al., 1983), mouse—human fusion partners (Kozbor and Roder, 1984, 1983b), and optimization of fusion protocols (Buck et al., 1984; Truitt et al., 1984) has slightly increased the frequency of specific antibodies, but the efficiency is still far less than that of immunized mice or rats. Even with a greater understanding of the postimmunization kinetics of immune B-cell precursors in peripheral human blood (Callard et al., 1982; Butler et al.,1983; Astaldi et al., 1982), production of antibody-producing human hybridomas is still an uncommon event.
Keywords
- Human Monoclonal Antibody
- Parent Cell Line
- Human Lymphoblastoid Cell Line
- Diphtheria Antitoxin
- Fusion Protocol
These keywords were added by machine and not by the authors. This process is experimental and the keywords may be updated as the learning algorithm improves.
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Larrick, J.W. et al. (1985). In Vitro Expansion of Human B Cells for the Production of Human Monoclonal Antibodies. In: Engleman, E.G., Foung, S.K.H., Larrick, J.W., Raubitschek, A.A. (eds) Human Hybridomas and Monoclonal Antibodies. Springer, Boston, MA. https://doi.org/10.1007/978-1-4684-4949-5_9
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DOI: https://doi.org/10.1007/978-1-4684-4949-5_9
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