AbstractAn easy and rapid isolation technique of human T cells on a polystyrene resin particle column has been developed. The cells of the effluent fraction contained more than 90 sheep erythrocyte (SRBC) rosette‐forming cells and less than 1 of cells bearing surface immunoglobulin (Ig) or peroxidase. The T cell (SRBC rosette‐forming cells) recovery rate was 80. The distribution of OKT antigen T cell subsets was essentially the same as that of T cells separated by rosette sedimentation. Cell functions such as tritiated thymidine uptake by T cells and helper activity in Ig production were also the same as that of T cells separated by SRBC rosette sedimentation. Natural killer‐like activity of the T cells isolated by the present method increased more than that of T cells obtained by the conventional method. Moreover, it was free from functional modification which tends to result from stimulation such as by the SRBC antigen in the SRBC centrifugation method. The combination of a T cell population offered by the present method and B cells depleted of SRBC‐binding B cells minimized background plaque formation and enabled us to quantify the plaque‐forming cell number in an antigen‐specific plaque‐forming assay. Furthermore, these populations produced relatively pure interleukin 2 (IL2) by stimulation of an autologous mixed lymphocyte reaction without any absorption of IL2 produced in the same culture. It seemed to be useful to evaluate the ability of lymphocytes from normal individuals and patients t
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