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白细胞介素-2在丝状噬菌体上的功能展示。

The functional display of interleukin-2 on filamentous phage.

作者信息

Buchli P J, Wu Z, Ciardelli T L

机构信息

Department of Pharmacology and Toxicology, Dartmouth Medical School, Hanover, New Hampshire 03755, USA.

出版信息

Arch Biochem Biophys. 1997 Mar 1;339(1):79-84. doi: 10.1006/abbi.1996.9853.

Abstract

We report the novel display of interleukin-2 (IL-2) and an IL-2 analog, D126, on the surface of filamentous bacteriophage using a phagemid vector system. A synthetic human IL-2 gene and its D126 analog were fused to the carboxyl-terminal domain of the gene III minor phage coat protein. Expression of IL-2 and D126 was verified by their reactivity with an IL-2-specific antibody. Biological response of IL-2 phage on murine CTLL-2 cells was comparable to that of recombinant soluble IL-2, while the D126 phage displayed a reduced biological response similar to that previously measured by soluble D126 protein. Biosensor surface plasmon resonance was employed to verify binding of the IL-2 and D126 phage to the IL-2 alpha beta cc receptor complex. A 41-fold enrichment of IL-2 phage over R408 helper phage was demonstrated in biopanning affinity selection studies employing biotinylated alpha beta cc receptor complex. These biopanning studies are the first reports of affinity selection of IL-2 phage and demonstrate a novel use for the alpha beta cc receptor complex. Together, these studies confirm that the structural integrity of IL-2 and D126 is maintained when they are displayed as a gIIIp fusion protein on phage particles and provide the foundation for further selection studies employing IL-2 analog phage libraries.

摘要

我们报道了使用噬菌粒载体系统在丝状噬菌体表面展示白细胞介素-2(IL-2)和一种IL-2类似物D126的新方法。将合成的人IL-2基因及其D126类似物与基因III小噬菌体外壳蛋白的羧基末端结构域融合。通过IL-2特异性抗体的反应性验证了IL-2和D126的表达。IL-2噬菌体对小鼠CTLL-2细胞的生物学反应与重组可溶性IL-2相当,而D126噬菌体表现出降低的生物学反应,类似于先前用可溶性D126蛋白测得的反应。采用生物传感器表面等离子体共振来验证IL-2和D126噬菌体与IL-2αβcc受体复合物的结合。在使用生物素化的αβcc受体复合物的生物淘选亲和选择研究中,证明IL-2噬菌体比R408辅助噬菌体富集了41倍。这些生物淘选研究是关于IL-2噬菌体亲和选择的首次报道,并证明了αβcc受体复合物的新用途。总之,这些研究证实,当IL-2和D126作为gIIIp融合蛋白展示在噬菌体颗粒上时,它们的结构完整性得以维持,并为进一步利用IL-2类似物噬菌体文库进行选择研究奠定了基础。

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