Gemlo B T, Palladino M A, Jaffe H S, Espevik T P, Rayner A A
Department of Surgery, University of California, San Francisco 94143.
Cancer Res. 1988 Oct 15;48(20):5864-7.
Treatment with recombinant interleukin 2 and lymphokine-activated killer cells (rIL-2/LAK) has produced a clinical antitumor effect in preliminary human trials. The cytokines gamma-interferon (IFN-gamma), tumor necrosis factor alpha (TNF-alpha), and tumor necrosis factor beta (TNF-beta, lymphotoxin) have potent in vitro antitumor activity and some clinical toxicities similar to interleukin 2 (IL-2)/LAK. This study sought to determine whether these cytokines were detectable in sera of IL-2/LAK-treated patients. Ten patients were treated with a protocol of 5-day i.v. rIL-2 bolus priming (10(5) units/kg, every 8 h), followed by 5 daily phereses with harvested lymphocytes cultured in vitro to generate LAK, and 5 days of rIL-2 bolus with infusion of LAK cells. Five patients were treated with a protocol modified to a 3-day rIL-2 prime and 6-day continuous infusion rIL-2 (3 x 10(6) units/m2/day) with infusion of LAK cells. Serum specimens were obtained prior to and 0.5, 2, 3, and 5 h after IL-2 or LAK cell administrations. IFN-gamma was detected by enzyme-linked immunosorbent assay, TNF-alpha by WEHI 164 bioassay or enzyme-linked immunosorbent assay, and TNF-beta by WEHI 164 cell bioassay. During the prime, few patients manifested in vivo detectable serum cytokines: IFN-gamma, three of ten, 5-day prime (1.03 +/- 0.46 ng/ml), and zero of five, 3-day prime; TNF-alpha, one of ten, 5-day prime, and one of three, 3-day prime; TNF-beta, one of ten, 5-day prime. The supernatants of in vitro LAK generation cultures had detectable levels of cytokines at 24 h which increased progressively until culture harvest at Day 4 (IFN-gamma, 2.56 +/- 0.34 ng/ml; TNF-alpha, 356 +/- 110 pg/ml; TNF-beta, 8.2 +/- 4.4 units/ml). The highest levels of in vivo serum cytokines occurred following LAK cell infusion and were more often elevated in patients receiving rIL-2 by bolus than by continuous infusion: IFN-gamma, four of six bolus, zero of three continuous infusion; TNF-alpha, six of six bolus (maximum 679 pg/ml) versus two of three continuous infusion (maximum, 106 pg/ml). LAK cells in vitro responded with cytokine release on stimulation by tumor cell lines (IFN-gamma, 0.88 +/- 0.06 ng/ml; TNF-alpha, 426 +/- 16 pg/ml; TNF-beta, 0.64 +/- 0.06 units/ml). In summary, this preliminary study has detected circulating cytokines in sera of patients receiving IL-2/LAK therapy. The greatest cytokine elevations followed LAK cell infusion.(ABSTRACT TRUNCATED AT 400 WORDS)
重组白细胞介素2与淋巴因子激活的杀伤细胞(rIL-2/LAK)治疗在初步人体试验中已产生临床抗肿瘤效果。细胞因子γ干扰素(IFN-γ)、肿瘤坏死因子α(TNF-α)和肿瘤坏死因子β(TNF-β,淋巴毒素)具有强大的体外抗肿瘤活性以及一些与白细胞介素2(IL-2)/LAK类似的临床毒性。本研究旨在确定在接受IL-2/LAK治疗的患者血清中是否可检测到这些细胞因子。10名患者接受了为期5天的静脉注射rIL-2大剂量启动方案(10⁵单位/千克,每8小时一次),随后连续5天进行每日一次的血细胞分离术,采集淋巴细胞并在体外培养以产生LAK,然后进行5天的rIL-2大剂量注射并输注LAK细胞。5名患者接受了修改后的方案,即3天的rIL-2启动和6天的rIL-2持续输注(3×10⁶单位/平方米/天)并输注LAK细胞。在给予IL-2或LAK细胞之前以及之后0.5、2、3和5小时采集血清标本。通过酶联免疫吸附测定法检测IFN-γ,通过WEHI 164生物测定法或酶联免疫吸附测定法检测TNF-α,通过WEHI 164细胞生物测定法检测TNF-β。在启动阶段,很少有患者体内可检测到血清细胞因子:IFN-γ,5天启动方案的10名患者中有3名(1.03±0.46纳克/毫升),3天启动方案的5名患者中为0名;TNF-α,5天启动方案的10名患者中有1名,3天启动方案的3名患者中有1名;TNF-β,5天启动方案的10名患者中有1名。体外LAK生成培养物的上清液在24小时时可检测到细胞因子水平,且在第4天培养收获前逐渐升高(IFN-γ,2.56±0.34纳克/毫升;TNF-α,356±110皮克/毫升;TNF-β,8.2±4.4单位/毫升)。体内血清细胞因子的最高水平出现在输注LAK细胞之后,且接受大剂量rIL-2的患者比接受持续输注的患者更常出现升高:IFN-γ,大剂量组6名患者中有4名,持续输注组3名患者中为0名;TNF-α,大剂量组6名患者中有6名(最高679皮克/毫升),持续输注组3名患者中有2名(最高106皮克/毫升)。体外LAK细胞在受到肿瘤细胞系刺激时会释放细胞因子(IFN-γ,0.88±0.06纳克/毫升;TNF-α,426±16皮克/毫升;TNF-β,0.64±0.06单位/毫升)。总之,这项初步研究在接受IL-2/LAK治疗的患者血清中检测到了循环细胞因子。细胞因子升高最明显的情况出现在输注LAK细胞之后。(摘要截短至400字)
