Murphy J R, Bishai W, Williams D, Bacha P, Borowski M, Parker K, Boyd J, Waters C, Strom T B
Evans Department of Clinical Research, University Hospital, Boston University Medical Center, MA 02115.
Biochem Soc Symp. 1987;53:9-23.
The reports of Miyanohara et al. (1986) and Murphy et al. (1986) were the first to describe the genetic construction, expression, and receptor-specific selective toxicity of a chimaeric toxin. In the present report, we have extended these earlier observations and have shown that the fusion of a modified gene encoding IL-2 to a truncated diphtheria toxin gene also results in the expression of a biologically active chimaeric IL-2 toxin. In both instances we have used receptor-binding-domain substitution and have genetically coupled those portions of the diphtheria toxin structural gene that encode the ADP-ribosyl transferase activity of fragment A and lipid-associating domains of fragment B to modified genes which encode either the polypeptide hormone alpha-MSH or the T-cell growth factor IL-2. The chimaeric toxins expressed from these gene fusions have been shown to be selectively targeted to those eukaryotic cells that carry specific surface receptors for the ligand compounds of the hybrid. For example, in the case of the IL-2 toxin, it is clear that the selective action of this hybrid protein is based upon both its diphtheria-toxin and IL-2-related components. Following binding to the IL-2R on activated and/or malignant T-cell, IL-2 toxin is internalized by receptor-mediated endocytosis. Upon acidification of the endosome, diphtheria toxin fragment B portions of the chimaeric toxin facilitate the delivery of fragment A to the cytosol where it catalyses the ADP ribosylation of EF-2. The assembly of chimaeric toxins at the level of the gene offers several advantages over chemical linkage. Since chemical linkage of the toxophore and ligand components of the conjugate toxins requires activation of the epsilon-amino moiety of lysine residues with reagents that will allow for subsequent disulphide linkage, the precise site of coupling is generally not known. In addition, there has been considerable concern over the lability of the disulphide bond between the toxophore and ligand components in vivo due to the action of disulphide reductases. The assembly of chimaeric toxins at the level of the gene allows for precise linkage of the toxophore and ligand components. Since the linkage between the toxophore and ligand is a peptide bond, the chimaeric toxin should be stable in vivo. In addition, the genetic construction of chimaeric toxins also allows for further protein engineering through site-directed mutagenesis.(ABSTRACT TRUNCATED AT 400 WORDS)
宫原等人(1986年)和墨菲等人(1986年)的报告首次描述了嵌合毒素的基因构建、表达及受体特异性选择毒性。在本报告中,我们扩展了这些早期观察结果,并表明将编码IL-2的修饰基因与截短的白喉毒素基因融合,也会导致具有生物活性的嵌合IL-2毒素的表达。在这两种情况下,我们都使用了受体结合域替换,并通过基因手段将白喉毒素结构基因中编码片段A的ADP-核糖基转移酶活性和片段B的脂质结合域的部分,与编码多肽激素α-MSH或T细胞生长因子IL-2的修饰基因相连接。已证明从这些基因融合体表达的嵌合毒素能选择性地作用于那些携带该杂种配体化合物特异性表面受体的真核细胞。例如,就IL-2毒素而言,很明显这种杂合蛋白的选择性作用基于其白喉毒素和IL-2相关成分。与活化的和/或恶性T细胞上的IL-2R结合后,IL-2毒素通过受体介导的内吞作用被内化。当内体酸化时,嵌合毒素的白喉毒素片段B部分促进片段A递送至胞质溶胶,在那里它催化EF-2的ADP核糖基化。在基因水平上组装嵌合毒素比化学连接具有几个优点。由于缀合毒素的毒素部分和配体成分的化学连接需要用能允许后续二硫键连接的试剂激活赖氨酸残基的ε-氨基部分,所以通常不知道精确的偶联位点。此外,由于二硫键还原酶的作用,毒素部分和配体成分之间的二硫键在体内的稳定性一直备受关注。在基因水平上组装嵌合毒素可实现毒素部分和配体成分的精确连接。由于毒素部分和配体之间的连接是肽键,嵌合毒素在体内应该是稳定的。此外,嵌合毒素的基因构建还允许通过定点诱变进行进一步的蛋白质工程改造。(摘要截选至400字)
