Our studies have analyzed pore-forming protein (PFP) mRNA expression in resting and stimulated human peripheral blood CD3- large granular lymphocytes (LGL), CD3+ T cells, and their CD4+ or CD8+ subsets. Signals that stimulate T cells to develop cytotoxic activity (i.e., IL-2 or OKT-3 mAb) led to the induction of PFP mRNA in T cells. The data indicated that IL-2 directly increased PFP mRNA in the CD8+ subset of T cells, in the absence of new DNA or protein synthesis. Abrogation of IL-2-induced PFP mRNA expression and cytotoxic potential of T cells by the anti-p75 IL-2 receptor mAb suggested that low numbers of p75 IL-2 receptors on CD8+ T cells were capable of transducing signals responsible for these IL-2-induced effects. The induction of T cell PFP mRNA via CD3, using OKT-3 mAb, was less rapid but greater than that caused by IL-2; however, a combination of PMA and ionomycin, which bypasses crosslinking of the TCR/CD3 complex, could not mimic this increase in PFP mRNA levels in T cells. The role of second messenger systems in regulating PFP mRNA expression remains to be determined. In contrast, high constitutive PFP mRNA expression was observed in CD3- LGL and these mRNA levels could not be enhanced by stimulation with IL-2. The cytotoxic potential of peripheral blood T cells and LGL induced in response to IL-2 correlated with IL-2-induced PFP mRNA levels in these cells and was consistent with PFP being one of several important molecules involved in the effector function of cytotoxic lymphocytes.
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1 April 1990
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April 01 1990
Interleukin 2 induction of pore-forming protein gene expression in human peripheral blood CD8+ T cells.
M J Smyth,
M J Smyth
Laboratory of Experimental Immunology, National Cancer Institute-Frederick Cancer Research Facility, Maryland 21701.
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J R Ortaldo,
J R Ortaldo
Laboratory of Experimental Immunology, National Cancer Institute-Frederick Cancer Research Facility, Maryland 21701.
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Y Shinkai,
Y Shinkai
Laboratory of Experimental Immunology, National Cancer Institute-Frederick Cancer Research Facility, Maryland 21701.
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H Yagita,
H Yagita
Laboratory of Experimental Immunology, National Cancer Institute-Frederick Cancer Research Facility, Maryland 21701.
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M Nakata,
M Nakata
Laboratory of Experimental Immunology, National Cancer Institute-Frederick Cancer Research Facility, Maryland 21701.
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K Okumura,
K Okumura
Laboratory of Experimental Immunology, National Cancer Institute-Frederick Cancer Research Facility, Maryland 21701.
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H A Young
H A Young
Laboratory of Experimental Immunology, National Cancer Institute-Frederick Cancer Research Facility, Maryland 21701.
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M J Smyth
Laboratory of Experimental Immunology, National Cancer Institute-Frederick Cancer Research Facility, Maryland 21701.
J R Ortaldo
Laboratory of Experimental Immunology, National Cancer Institute-Frederick Cancer Research Facility, Maryland 21701.
Y Shinkai
Laboratory of Experimental Immunology, National Cancer Institute-Frederick Cancer Research Facility, Maryland 21701.
H Yagita
Laboratory of Experimental Immunology, National Cancer Institute-Frederick Cancer Research Facility, Maryland 21701.
M Nakata
Laboratory of Experimental Immunology, National Cancer Institute-Frederick Cancer Research Facility, Maryland 21701.
K Okumura
Laboratory of Experimental Immunology, National Cancer Institute-Frederick Cancer Research Facility, Maryland 21701.
H A Young
Laboratory of Experimental Immunology, National Cancer Institute-Frederick Cancer Research Facility, Maryland 21701.
Online ISSN: 1540-9538
Print ISSN: 0022-1007
J Exp Med (1990) 171 (4): 1269–1281.
Citation
M J Smyth, J R Ortaldo, Y Shinkai, H Yagita, M Nakata, K Okumura, H A Young; Interleukin 2 induction of pore-forming protein gene expression in human peripheral blood CD8+ T cells.. J Exp Med 1 April 1990; 171 (4): 1269–1281. doi: https://doi.org/10.1084/jem.171.4.1269
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