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在转基因烟草中进行人类酶的生物生产。

Bioproduction of human enzymes in transgenic tobacco.

作者信息

Cramer C L, Weissenborn D L, Oishi K K, Grabau E A, Bennett S, Ponce E, Grabowski G A, Radin D N

机构信息

CropTech Development Corp. Virginia Tech Corporate Research Center, Blacksburg 24060, USA.

出版信息

Ann N Y Acad Sci. 1996 May 25;792:62-71. doi: 10.1111/j.1749-6632.1996.tb32492.x.

Abstract

Transgenic plants have significant potential in the bioproduction of complex human therapeutic proteins due to ease of genetic manipulation, lack of potential contamination with human pathogens, conservation of eukaryotic cell machinery mediating protein modification, and low cost of biomass production. Tobacco has been used as our initial transgenic system because Agrobacterium-mediated transformation is highly efficient, prolific seed production greatly facilitates biomass scale-up, and development of new "health-positive" uses for tobacco has significant regional support. We have targeted bioproduction of complex recombinant human proteins with commercial potential as human pharmaceuticals. Human protein C (hPC), a highly processed serum protease of the coagulation/anticoagulation cascade, was produced at low levels in transgenic tobacco leaves. Analogous to its processing in mammalian systems, tobacco-synthesized hPC appears to undergo multiple proteolytic cleavages, disulfide bond formation, and N-linked glycosylation. Although tobacco-derived hPC has not yet been tested for all posttranslational modifications or for enzymatic (anticlotting) activity, these results are promising and suggest considerable conservation of protein processing machinery between plants and animals. CropTech researchers have also produced the human lysosomal enzyme glucocerebrosidase (hGC) in transgenic tobacco. This glycoprotein has significant commercial potential as replacement therapy in patients with Gaucher's disease. Regular intravenous administration of modified glucocerebrosidase, derived from human placentae or CHO cells, has proven highly effective in reducing disease manifestations in patients with Gaucher's disease. However, the enzyme is expensive (dubbed the "world's most expensive drug" by the media), making it a dramatic model for evaluating the potential of plants to provide a safe, low-cost source of bioactive human enzymes. Transgenic tobacco plants were generated that contained the human glucocerebrosidase cDNA under the control of an inducible plant promoter. hGC expression was demonstrated in plant extracts by enzyme activity assay and immunologic cross-reactivity with anti-hGC antibodies. Tobacco-synthesized hGC comigrates with human placental-derived hGC during electrophoretic separations, is glycosylated, and, most significantly, is enzymatically active. Although expression levels vary depending on transformant and induction protocol, hGC production of > 1 mg/g fresh weight of leaf tissue has been attained in crude extracts. Our studies provide strong support for the utilization of tobacco for high-level production of active hGC for purification and eventual therapeutic use at potentially much reduced costs. Furthermore, this technology should be directly adaptable to the production of a variety of other complex human proteins of biologic and pharmaceutical interest.

摘要

由于易于进行基因操作、不存在被人类病原体污染的潜在风险、介导蛋白质修饰的真核细胞机制得以保留以及生物质生产成本较低,转基因植物在复杂人类治疗性蛋白质的生物生产中具有巨大潜力。烟草已被用作我们最初的转基因系统,因为农杆菌介导的转化效率很高,大量的种子生产极大地促进了生物质的扩大,并且烟草新的“对健康有益”用途的开发得到了重要的区域支持。我们的目标是生物生产具有作为人类药物商业潜力的复杂重组人类蛋白质。人蛋白C(hPC)是凝血/抗凝级联反应中一种经过高度加工的血清蛋白酶,在转基因烟草叶片中的产量较低。与它在哺乳动物系统中的加工过程类似,烟草合成的hPC似乎经历了多次蛋白水解切割、二硫键形成和N-糖基化。尽管源自烟草的hPC尚未针对所有翻译后修饰或酶活性(抗凝血)进行测试,但这些结果很有前景,表明植物和动物之间的蛋白质加工机制有相当程度的保守性。作物技术研究人员还在转基因烟草中生产了人类溶酶体酶葡萄糖脑苷脂酶(hGC)。这种糖蛋白作为戈谢病患者的替代疗法具有巨大的商业潜力。定期静脉注射源自人胎盘或CHO细胞的修饰葡萄糖脑苷脂酶,已被证明在减轻戈谢病患者的疾病症状方面非常有效。然而,这种酶价格昂贵(被媒体称为“世界上最昂贵的药物”),这使其成为评估植物提供安全、低成本生物活性人类酶来源潜力的一个典型例子。构建了在可诱导植物启动子控制下含有人类葡萄糖脑苷脂酶cDNA的转基因烟草植株。通过酶活性测定和与抗hGC抗体的免疫交叉反应,在植物提取物中证实了hGC的表达。在电泳分离过程中,烟草合成的hGC与人胎盘来源的hGC迁移情况相同,具有糖基化,并且最显著的是具有酶活性。尽管表达水平因转化体和诱导方案而异,但在粗提取物中已实现每克叶组织鲜重产生超过1毫克的hGC产量。我们的研究为利用烟草高水平生产活性hGC以进行纯化并最终以可能大幅降低的成本用于治疗提供了有力支持。此外,这项技术应该可以直接应用于生产多种其他具有生物学和药学意义的复杂人类蛋白质。

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