Pearson J W, Hedrick E, Fogler W E, Bull R L, Ferris D K, Riggs C W, Wiltrout R H, Sivam G, Morgan A C, Groves E
Biological Response Modifiers Program, NCI-FCRDC, Maryland 21702-1201.
Cancer Res. 1990 Oct 1;50(19):6379-88.
The antitumor effects of two immunotoxins were evaluated in vitro and in vivo against the human ovarian carcinoma cell line, OVCAR-3. The immunotoxins used were composed of recombinant ricin A chain (rRTA) covalently attached to a monoclonal antibody directed toward the human transferrin receptor (45412/rRTA, also called 454A12 MAB-rRTA by Cetus Corporation) or Pseudomonas exotoxin coupled to an anticarcinoma monoclonal antibody (NR-LU-10/PE). Preliminary characterization of the NR-LU-10 antigen by immunoprecipitation and cellular fluorescence demonstrated two dominant cell surface polypeptide moieties with molecular weights of 40,000 and 45,000 and a minor component with a molecular weight of 33,000. The immunotoxins were used alone or in combination with recombinant human alpha-interferon (rhIFN-alpha). Protein synthesis was inhibited in a dose-dependent manner in OVCA-3 cells incubated in vitro with either NR-LU-10/PE or 454A12/rRTA (50% inhibitory concentrations, 1 and 75 ng/ml, respectively). Unconjugated NR-LU-10 or 454A12 abrogated the activity of the relevant immunotoxins. Concomitant incubation in vitro of OVCAR-3 cells with NR-LU-10/PE or 454A12/rRTA and a noncytotoxic concentration of rhIFN-alpha potentiated the inhibitory activity of the immunotoxins via a mechanism independent of antigenic upregulation. This potentially synergistic combination was then tested in vivo. The median survival time (MST) of mice given injections i.p. of 4 x 10(6) OVCAR-3 cells was 46 days. Cohorts of mice that received intracavitary treatment beginning 5 days posttumor cell inoculation with either 0.25 or 0.5 microgram of NR-LU-10/PE every other day for a total of 10 treatments exhibited a significantly increased MST of 63 and 104 days, respectively (P less than 0.0001). Likewise, the i.p. injection of either 2.5 or 10 micrograms of 454A12/rRTA given in an identical schedule resulted in a MST of 89 and greater than 120 days, respectively (P less than 0.0001). When rhIFN-alpha was administered i.p. in conjunction with those doses of either immunotoxin, a significant increase in the MST was observed in comparison with mice given immunotoxin alone. The combination of 5 x 10(4) units of rhIFN-alpha and 0.25 microgram of NR-LU-10/PE resulted in 67% long-term survivors (greater than 120 days) compared with only 13% survival of mice given the immunotoxin alone. Similarly, 2.5 micrograms of 454A12/rRTA plus rhIFN-alpha resulted in an enhanced therapeutic response (89% long-term survivors) when compared with 454A12/rRTA alone (29%).(ABSTRACT TRUNCATED AT 400 WORDS)
在体外和体内评估了两种免疫毒素对人卵巢癌细胞系OVCAR-3的抗肿瘤作用。所使用的免疫毒素由与针对人转铁蛋白受体的单克隆抗体共价连接的重组蓖麻毒素A链(rRTA)组成(45412/rRTA,Cetus公司也称为454A12 MAB-rRTA)或与抗癌单克隆抗体偶联的铜绿假单胞菌外毒素(NR-LU-10/PE)。通过免疫沉淀和细胞荧光对NR-LU-10抗原进行的初步表征显示,有两个主要的细胞表面多肽部分,分子量分别为40,000和45,000,还有一个分子量为33,000的次要成分。免疫毒素单独使用或与重组人α干扰素(rhIFN-α)联合使用。在体外与NR-LU-10/PE或454A12/rRTA孵育的OVCA-3细胞中,蛋白质合成以剂量依赖性方式受到抑制(50%抑制浓度分别为1和75 ng/ml)。未偶联的NR-LU-10或454A12消除了相关免疫毒素的活性。OVCAR-3细胞在体外与NR-LU-10/PE或454A12/rRTA以及无细胞毒性浓度的rhIFN-α共同孵育,通过一种独立于抗原上调的机制增强了免疫毒素的抑制活性。然后在体内测试了这种潜在的协同组合。腹腔注射4×10⁶个OVCAR-3细胞的小鼠的中位生存时间(MST)为46天。在肿瘤细胞接种后5天开始接受腔内治疗的小鼠队列,每隔一天注射0.25或0.5微克NR-LU-10/PE,共进行10次治疗,其MST分别显著增加至63天和104天(P<0.0001)。同样,按照相同方案腹腔注射2.5或10微克454A12/rRTA,MST分别为89天和大于120天(P<0.0001)。当rhIFN-α与这些剂量的任何一种免疫毒素联合腹腔给药时,与单独给予免疫毒素的小鼠相比,MST显著增加。5×10⁴单位的rhIFN-α与0.25微克NR-LU-10/PE联合使用,导致67%的长期存活者(大于120天),而单独给予免疫毒素的小鼠存活率仅为13%。同样,与单独使用454A12/rRTA(29%)相比,2.5微克454A12/rRTA加rhIFN-α导致治疗反应增强(89%长期存活者)。(摘要截短于400字)
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