Lamers C H J, van Elzakker P, Langeveld S C L, Sleijfer S, Gratama J W
Unit Clinical and Tumor Immunology, Department of Medical Oncology, Erasmus University Medical Center-Daniel den Hoed Cancer Center, Rotterdam, the Netherlands.
Cytotherapy. 2006;8(6):542-53. doi: 10.1080/14653240601056396.
Adoptive transfer of autologous T cells that are gene-transduced to express Ag-specific receptors represents an experimental strategy to provide tumor-specific immunity to cancer patients. We studied this concept in patients with metastatic renal cell cancer (RCC) using retroviral transduction of T cells with a single-chain Ab-G250 chimeric receptor [scFv(G250)]. We describe the validation of our clinical protocol for gene transduction and expansion of human T lymphocytes.
A batch of scFv(G250) transgene-containing retrovirus was produced under conditions of good manufacturing practice (GMP). In addition to quality control and safety testing of the virus batch, extensive potency testing was performed, i.e. assessment of its functional transduction efficiency in primary human T cells. Subsequently, the clinical gene transduction and cell-expansion protocol was subjected to a series of process validations and a clinical evaluation using T cells obtained from healthy donors and three RCC patients.
The clinical batch of scFv(G250) transgene-containing retrovirus met the quality and safety control criteria. Small-scale transductions yielded 62-92% scFv(G250)+ T cells and, at a clinical scale, 50-84% transduction efficiencies were obtained. Patient and healthy donor T cells showed similar expansion potencies, and also yielded similar levels of scFv(G250)-mediated immune functions, i.e. specific cytolysis of G250-ligand expressing RCC cells and production of IFN-gamma upon stimulation with such cells. All T cell cultures were free of replication competent retroviruses.
We have shown that the validated batch of scFv(G250) transgene-containing retrovirus in combination with our GMP T-cell transduction and expansion protocol successfully generates clinically relevant numbers of functional scFv(G250) gene-modified T cells for patient treatment.
采用基因转导以表达抗原特异性受体的自体T细胞进行过继性转移,是为癌症患者提供肿瘤特异性免疫的一种实验策略。我们利用单链抗体-G250嵌合受体[scFv(G250)]对T细胞进行逆转录病毒转导,在转移性肾细胞癌(RCC)患者中研究了这一概念。我们描述了用于人类T淋巴细胞基因转导和扩增的临床方案的验证情况。
在良好生产规范(GMP)条件下生产一批含scFv(G250)转基因的逆转录病毒。除了对病毒批次进行质量控制和安全性检测外,还进行了广泛的效价检测,即评估其在原代人T细胞中的功能转导效率。随后,使用从健康供体和三名RCC患者获得的T细胞,对临床基因转导和细胞扩增方案进行了一系列工艺验证和临床评估。
临床批次的含scFv(G250)转基因的逆转录病毒符合质量和安全控制标准。小规模转导产生了62%-92%的scFv(G250)+T细胞,在临床规模下,转导效率为50%-84%。患者和健康供体的T细胞显示出相似的扩增能力,并且产生的scFv(G250)介导的免疫功能水平也相似,即对表达G250配体的RCC细胞的特异性细胞溶解作用,以及在用此类细胞刺激后产生γ干扰素。所有T细胞培养物均无具有复制能力的逆转录病毒。
我们已经证明,经验证的含scFv(G250)转基因的逆转录病毒批次,与我们的GMP T细胞转导和扩增方案相结合,成功地产生了临床上相关数量的功能性scFv(G250)基因修饰的T细胞用于患者治疗。
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