Ram Z, Culver K W, Walbridge S, Frank J A, Blaese R M, Oldfield E H
Surgical Neurology Branch, National Institute of Neurological Disorders and Stroke, National Institutes of Health, Bethesda, Maryland.
J Neurosurg. 1993 Sep;79(3):400-7. doi: 10.3171/jns.1993.79.3.0400.
Retroviral-mediated transfer of the herpes simplex virus thymidine kinase (HSVtk) gene into malignant tumors confers drug susceptibility to the antiviral drug ganciclovir. The authors have recently shown that in situ transduction of the rat 9L brain tumor following HSVtk-producer cell implantation led to tumor regression after ganciclovir administration in treated rats. A wide spectrum of potential adverse effects may, however, be associated with the application of this approach to treat brain tumors, including dissemination of the retroviral vector to nontumoral tissues within or outside the central nervous system, proliferation of the injected murine vector-producer cells at the injection site, immune-mediated responses to the implantation of xenogeneic cells, and damage to the brain from toxic by-products of the HSVtk-ganciclovir interaction. These possibilities were investigated using intracerebral and systemic injections of retroviral vector-producer cells carrying the HSVtk or the lacZ gene in mice, rats, and nonhuman primates. Using the lacZ gene as a reporter gene, no evidence of beta-galactosidase activity consistent with vector transduction was detected in any major body organ in the treated mice or rats. Similarly, the HSVtk gene transfer did not result in toxicity, with or without ganciclovir administration. In studies using rat and monkey models, no proliferation of the vector-producer cells occurred after intracerebral injection. Vector-producer cell survival was limited to 7 to 14 days. High-dose steroid therapy did not appear to extend the survival of these xenogeneic cells in rats. No significant inflammatory response was observed in the meninges or brain parenchyma. Endothelial cells were occasionally transduced in brain capillaries adjacent to the injected site of the vector-producer cells. Injection of producer cells into brain tissue elicited mild edema and reactive gliosis surrounding the injection site, which were probably the cause of a transient toxic response arising 4 to 5 days following injection of the producer cells; short-term administration of dexamethasone eliminated that response. No neurological deficits were observed in the rats or primates treated with the HSVtk vector-producer cells, with or without ganciclovir. In primates injected with producer cells, magnetic resonance imaging before, during, and after ganciclovir administration showed minimal and localized breakdown of the blood-brain barrier without significant edema or mass effect. Similarly, histological examination of the monkeys' brains showed no damage to neurons, astroglia, or myelin. Long-term clinical (> 9 months) and radiological (3 months) assessment of the primates has revealed no evidence of toxicity.(ABSTRACT TRUNCATED AT 400 WORDS)
逆转录病毒介导的单纯疱疹病毒胸苷激酶(HSVtk)基因转移至恶性肿瘤可使肿瘤对抗病毒药物更昔洛韦产生药物敏感性。作者最近表明,在植入HSVtk产生细胞后对大鼠9L脑肿瘤进行原位转导,在给治疗的大鼠施用更昔洛韦后导致肿瘤消退。然而,应用这种方法治疗脑肿瘤可能会产生广泛的潜在不良反应,包括逆转录病毒载体扩散到中枢神经系统内外的非肿瘤组织、注射的鼠源载体产生细胞在注射部位增殖、对异种细胞植入的免疫介导反应以及HSVtk-更昔洛韦相互作用的有毒副产物对脑的损害。使用携带HSVtk或lacZ基因的逆转录病毒载体产生细胞进行脑内和全身注射,在小鼠、大鼠和非人灵长类动物中对这些可能性进行了研究。使用lacZ基因作为报告基因,在接受治疗的小鼠或大鼠的任何主要身体器官中均未检测到与载体转导一致的β-半乳糖苷酶活性证据。同样,无论是否施用更昔洛韦,HSVtk基因转移均未导致毒性。在使用大鼠和猴子模型的研究中,脑内注射后载体产生细胞未发生增殖。载体产生细胞的存活期限于7至14天。高剂量类固醇疗法似乎并未延长这些异种细胞在大鼠中的存活期。在脑膜或脑实质中未观察到明显的炎症反应。在与载体产生细胞注射部位相邻的脑毛细血管中,偶尔会转导内皮细胞。将产生细胞注射到脑组织中会在注射部位周围引发轻度水肿和反应性胶质增生,这可能是注射产生细胞后4至5天出现短暂毒性反应的原因;短期给予地塞米松可消除该反应。在用HSVtk载体产生细胞治疗的大鼠或灵长类动物中,无论是否使用更昔洛韦,均未观察到神经功能缺损。在注射产生细胞的灵长类动物中,在施用更昔洛韦之前、期间和之后进行的磁共振成像显示血脑屏障仅有轻微的局部破坏,无明显水肿或占位效应。同样,对猴子大脑的组织学检查显示神经元、星形胶质细胞或髓鞘均未受损。对灵长类动物进行的长期临床(>9个月)和放射学(3个月)评估未发现毒性证据。(摘要截断于400字)
