Foon K A, Sen G, Hutchins L, Kashala O L, Baral R, Banerjee M, Chakraborty M, Garrison J, Reisfeld R A, Bhattacharya-Chatterjee M
Department of Internal Medicine, Lucille Parker Markey Cancer Center, University of Kentucky Medical Center, Lexington 40536-0093, USA.
Clin Cancer Res. 1998 May;4(5):1117-24.
We initiated a clinical trial for patients with advanced malignant melanoma treated with an anti-idiotype antibody that mimics the disialoganglioside GD2. We report the clinical and immune responses of the first 12 patients entered into this trial. Patients received 1-, 2-, 4-, or 8-mg doses of the anti-idiotype antibody mixed with 100 microg of QS-21 adjuvant every other week, four times, and then monthly. Twelve patients have been on trial for 2-23 months, and all of them have generated immune responses. Patients were removed from the study if they demonstrated disease progression. Hyperimmune sera from all 12 patients revealed an anti-anti-idiotypic Ab3 response, as demonstrated by the inhibition of Ab2 binding to Ab1 by patients' immune sera. To further test the anti-anti-idiotypic response, patients' Ab3 antibodies were affinity purified on Sepharose 4B columns containing adsorbed immunizing anti-idiotype immunoglobulin. Purified Ab3 of all patients studied inhibited binding of Ab1 to a GD2-positive cell line. Purified Ab3 also inhibited binding of Ab1 to purified GD2, in a manner comparable to equal quantities of purified Ab1. The patient Ab3 was truly an Ab1' because it specifically bound to purified disialoganglioside GD2. The isotypic specificity of the Ab3 antibody was predominantly IgG, with only minimal IgM. The predominant IgG subclass was IgG1, with approximately equal quantities of IgG2, IgG3, and IgG4. These Ab3 antibodies reacted specifically with tumor cells expressing GD2 by immune flow cytometry and immunoperoxidase assays. Five patients' Ab3 antibodies studied for antibody-dependent cellular cytotoxicity were positive. One patient had a complete clinical response, with resolution of soft tissue disease, and six patients had stable disease, ranging from 9 to 23 months, and are being continued on vaccine therapy. Toxicity consisted of local reaction at the site of the injection, including induration and pain that generally resolved within a few days. Mild fever and chills were observed in 75% of the patients but rarely required acetaminophen. There was no additional toxicity, including abdominal pain that was previously seen with infusion of murine monoclonal anti-GD2 antibody. Current trials include patients with stage III melanoma and small cell lung cancer. Future trials will attempt to enhance the antitumor response by the addition of interleukin 2, granulocyte macrophage colony-stimulating factor, and other cytokines, together with the 1A7 vaccine.
我们启动了一项针对晚期恶性黑色素瘤患者的临床试验,这些患者接受一种模拟双唾液酸神经节苷脂GD2的抗独特型抗体治疗。我们报告了进入该试验的前12名患者的临床和免疫反应。患者每隔一周接受1毫克、2毫克、4毫克或8毫克剂量的抗独特型抗体与100微克QS - 21佐剂混合,共四次,然后每月一次。12名患者已接受试验2至23个月,他们均产生了免疫反应。如果患者出现疾病进展,则将其从研究中剔除。所有12名患者的超免疫血清均显示出抗抗独特型Ab3反应,患者免疫血清对Ab2与Ab1结合的抑制作用证明了这一点。为了进一步检测抗抗独特型反应,将患者的Ab3抗体在含有吸附免疫抗独特型免疫球蛋白的琼脂糖4B柱上进行亲和纯化。所有研究患者的纯化Ab3均抑制Ab1与GD2阳性细胞系的结合。纯化的Ab3也以与等量纯化Ab1相当的方式抑制Ab1与纯化GD2的结合。患者的Ab3确实是一种Ab1',因为它能特异性结合纯化的双唾液酸神经节苷脂GD2。Ab3抗体的同种型特异性主要为IgG,仅有少量IgM。主要的IgG亚类是IgG1,IgG2、IgG3和IgG4的量大致相等。通过免疫流式细胞术和免疫过氧化物酶测定,这些Ab3抗体与表达GD2的肿瘤细胞发生特异性反应。研究的5名患者的Ab3抗体在抗体依赖性细胞毒性方面呈阳性。1名患者有完全的临床反应,软组织疾病消退,6名患者病情稳定,持续时间为9至23个月,目前仍在接受疫苗治疗。毒性反应包括注射部位的局部反应,包括硬结和疼痛,通常在几天内消退。75%的患者出现轻度发热和寒战,但很少需要使用对乙酰氨基酚。没有出现其他毒性反应,包括之前输注鼠源单克隆抗GD2抗体时所见的腹痛。目前的试验包括III期黑色素瘤和小细胞肺癌患者。未来的试验将尝试通过添加白细胞介素2、粒细胞巨噬细胞集落刺激因子和其他细胞因子以及1A7疫苗来增强抗肿瘤反应。
