Use of a SCID mouse/human lymphoma model to evaluate cytokine-induced killer cells with potent antitumor cell activity

I G Schmidt-Wolf, R S Negrin, H P Kiem, K G Blume, I L Weissman, I G Schmidt-Wolf, R S Negrin, H P Kiem, K G Blume, I L Weissman

Abstract

C.B-17 severe combined immune deficient (SCID) mice, which lack functional B and T lymphocytes, allow xenografts and, therefore, can be used to study the biology of human malignancies. Two different human B cell lymphoma cell lines, SU-DHL-4 and OCI-Ly8, which both harbor the t(14;18) chromosomal translocation, were injected into C.B-17 SCID mice. Mice injected intravenously or intraperitoneally developed tumors and died in a dose-dependent manner. The presence of tumor cells in various murine tissues could be demonstrated by a clonogenic tumor assay, staining of frozen sections with a monoclonal antibody (mAb) against a human B cell antigen (CD19), and with the polymerase chain reaction technique. A protocol using cytotoxic effector cells was developed and used to selectively deplete the tumor cells from bone marrow. These cells were developed by growing peripheral blood mononuclear cells in the presence of interferon gamma (IFN-gamma), anti-CD3 mAb, and interleukin 2 (IL-2). The timing of IFN-gamma treatment was critical and optimal if IFN-gamma was added before IL-2 treatment. The cells that were stimulated by IFN-gamma, followed by IL-2, could be expanded by treatment with a mAb directed against CD3. These cells could be further activated by IL-1, but not by tumor necrosis factor alpha. With this protocol, a tumor cell kill of 3 logs was obtained as measured by a clonogenic assay. Interestingly, despite their high cytotoxic activity against lymphoma cells, these cells had little toxicity against a subset of normal human hematopoietic precursor cells (granulocyte/macrophage colony-forming units). These cells were further tested by treating murine bone marrow contaminated with the human lymphoma cell line SU-DHL-4, and injecting these cells into SCID mice to assay for tumor growth in vivo. The animals injected with bone marrow contaminated with SU-DHL-4 cells had enhanced survival if the bone marrow was treated with the cytokine-induced killer cells before infusion. The SCID mouse provides a useful in vivo model for evaluation of new therapeutic approaches for lymphoma treatment. The cytokine-induced killer cells generated as described here could have an important impact on bone marrow purging for autologous bone marrow transplantation as well as for adoptive immunotherapy.

References

    1. Cell. 1986 Sep 26;46(7):963-72
    1. Am J Pathol. 1985 Sep;120(3):464-77
    1. Eur J Immunol. 1987 Jul;17(7):1051-7
    1. J Immunol. 1987 Apr 15;138(8):2728-33
    1. Int J Cancer. 1986 May 15;37(5):787-93
    1. Curr Top Microbiol Immunol. 1989;152:219-24
    1. Blood. 1989 Oct;74(5):1537-44
    1. J Immunol. 1985 Apr;134(4):2276-80
    1. Immunol Today. 1989 Oct;10(10):322-5
    1. J Immunol. 1989 Dec 15;143(12):4282-6
    1. J Immunol Methods. 1989 Dec 20;125(1-2):185-9
    1. Science. 1989 Dec 22;246(4937):1597-600
    1. Curr Top Microbiol Immunol. 1989;152:259-63
    1. Blood. 1987 May;69(5):1307-14
    1. Science. 1988 Sep 23;241(4873):1632-9
    1. Nature. 1988 Sep 15;335(6187):256-9
    1. J Immunol. 1985 May;134(5):3124-9
    1. Prog Exp Tumor Res. 1988;32:213-26
    1. Exp Hematol. 1988 Feb;16(2):131-8
    1. Blood. 1989 Jul;74(1):354-60
    1. Science. 1988 Dec 23;242(4886):1684-6
    1. J Clin Apher. 1988;4(2-3):113-7
    1. Important Adv Oncol. 1986;:55-91
    1. J Immunol Methods. 1987 Aug 24;102(1):127-41
    1. Cancer Res. 1986 Oct;46(10):4973-8
    1. Science. 1986 Sep 19;233(4770):1318-21
    1. J Immunol. 1986 Nov 1;137(9):2735-9
    1. Cancer Res. 1987 May 1;47(9):2456-60
    1. J Immunol. 1987 Apr 1;138(7):2338-44
    1. N Engl J Med. 1985 Dec 5;313(23):1485-92
    1. J Immunol. 1985 Jun;134(6):3798-801
    1. J Exp Med. 1990 Sep 1;172(3):985-8
    1. J Invest Dermatol. 1990 Mar;94(3):381-4
    1. Science. 1990 Feb 2;247(4942):564-6
    1. J Histochem Cytochem. 1984 Feb;32(2):219-29
    1. J Exp Med. 1982 Jun 1;155(6):1823-41
    1. J Immunol. 1984 Sep;133(3):1339-45
    1. J Immunol. 1984 Aug;133(2):1028-36
    1. J Immunol. 1984 Feb;132(2):787-95
    1. Nature. 1983 Feb 10;301(5900):527-30
    1. J Exp Med. 1978 Sep 1;148(3):714-26
    1. Blood. 1991 Feb 1;77(3):654-60
    1. J Mol Evol. 1986;23(1):11-22

Source: PubMed

Sponsorer og samarbeidspartnere

Medisinsk tilstand

Legemiddelintervensjoner

3
Abonnere