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外源性白细胞介素2通过体内活化的淋巴细胞募集体外淋巴因子激活的杀伤活性。

Exogenous interleukin 2 recruits in vitro lymphokine-activated killer activity by in vivo activated lymphocytes.

作者信息

Lamers H J, Gratama J W, van Putten W L, Stoter G, Bolhuis R L

机构信息

Department of Immunology, Dr. Daniel den Hoed Cancer Center, Rotterdam, The Netherlands.

出版信息

Cancer Res. 1991 May 1;51(9):2324-8.

PMID:2015597
Abstract

Cryopreserved and thawed lymphocytes can be used instead of fresh lymphocytes to avoid test-to-test variability in studies of fluctuations of natural killer (NK) and lymphokine-activated killer (LAK) activities as a function of time. We investigated the effects of 1-h versus 18-h resting of lymphocytes on their lytic activities, because the process of cryopreservation and thawing decreases NK and LAK activities. Lymphocytes from renal cell cancer patients receiving adoptive immunotherapy were studied. An 18-h versus 1-h resting period led to a significant increase in NK activity but had no significant effect on LAK activity. The presence of 1200 IU/ml interleukin 2 (IL-2) in the medium 1 h prior to and during the cytotoxicity (CTX) assay increased in vivo and in vitro IL-2-induced LAK activities. This phenomenon has been interpreted as IL-2 dependency of effector lymphocytes (J.A. Hank, P.C. Kohler, G. Weil-Hillman, N. Rosenthal, K. H. Moore, B. Storer, D. Minkoff, J. Bradshaw, R. Bechhofer, and P. M. Sondel. Cancer Res., 48: 1965-1971, 1988). We performed kinetic studies to assess the role of effector lymphocyte recruitment in these experiments. LAK activity was tested in the presence or absence of IL-2 during preincubations and CTX assays varying between 0 and 120 min. These kinetic studies showed that effector lymphocyte recruitment indeed contributed to the increased level of LAK activity when IL-2 was added to the CTX assay. A minimal incubation period of 30 min was required to detect recruitment of lymphocytes. Effector lymphocytes could be recruited for periods varying between 90 and greater than 240 min, depending on the lymphocyte donor. We conclude that: (a) in vitro, IL-2-mediated recruitment of lymphocytes due to presence of IL-2 in the CTX assay may lead to an overestimate of the actual LAK activity; and (b) in vivo, prolonged IL-2 infusion after the administration of activated lymphocytes seems warranted in order to recruit maximal levels of effector lymphocytes with LAK activity.

摘要

冷冻保存和解冻后的淋巴细胞可替代新鲜淋巴细胞,以避免在研究自然杀伤(NK)和淋巴因子激活的杀伤(LAK)活性随时间波动的实验中出现批次间差异。我们研究了淋巴细胞静置1小时与18小时对其裂解活性的影响,因为冷冻保存和解冻过程会降低NK和LAK活性。对接受过继性免疫治疗的肾细胞癌患者的淋巴细胞进行了研究。与静置1小时相比,静置18小时可使NK活性显著增加,但对LAK活性无显著影响。在细胞毒性(CTX)试验前1小时及试验期间,培养基中存在1200 IU/ml白细胞介素2(IL-2)可增加体内和体外IL-2诱导的LAK活性。这一现象被解释为效应淋巴细胞对IL-2的依赖性(J.A. Hank、P.C. Kohler、G. Weil-Hillman、N. Rosenthal、K.H. Moore、B. Storer、D. Minkoff、J. Bradshaw、R. Bechhofer和P.M. Sondel。《癌症研究》,48: 1965 - 1971,1988)。我们进行了动力学研究,以评估效应淋巴细胞募集在这些实验中的作用。在预孵育和持续时间在0至120分钟之间变化的CTX试验中,分别在有或无IL-2的情况下测试LAK活性。这些动力学研究表明,当在CTX试验中添加IL-2时,效应淋巴细胞募集确实有助于提高LAK活性水平。检测淋巴细胞募集需要至少30分钟的孵育期。根据淋巴细胞供体的不同,效应淋巴细胞可被募集90至超过240分钟不等。我们得出以下结论:(a)在体外,CTX试验中由于存在IL-2导致的IL-2介导的淋巴细胞募集可能会导致对实际LAK活性的高估;(b)在体内为了募集具有LAK活性的效应淋巴细胞达到最大水平,在给予活化淋巴细胞后延长IL-2输注时间似乎是必要的。

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