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与白喉毒素氨基末端融合的肽被转运到细胞质中。

Peptides fused to the amino-terminal end of diphtheria toxin are translocated to the cytosol.

作者信息

Stenmark H, Moskaug J O, Madshus I H, Sandvig K, Olsnes S

机构信息

Institute for Cancer Research, Norwegian Radium Hospital, Oslo.

出版信息

J Cell Biol. 1991 Jun;113(5):1025-32. doi: 10.1083/jcb.113.5.1025.

Abstract

Diphtheria toxin belongs to a group of toxic proteins that enter the cytosol of animal cells. We have here investigated the effect of NH2-terminal extensions of diphtheria toxin on its ability to become translocated to the cytosol. DNA fragments encoding peptides of 12-30 amino acids were fused by recombinant DNA technology to the 5'-end of the gene for a mutant toxin. The resulting DNA constructs were transcribed and translated in vitro. The translation products were bound to cells and then exposed to low pH to induce translocation across the cell membrane. Under these conditions all of the oligopeptides tested, including three viral peptides and the leader peptide of diphtheria toxin, were translocated to the cytosol along with the enzymatic part (A-fragment) of the toxin. Neither hydrophobic nor highly charged sequences blocked translocation. The results are compatible with a model in which the COOH-terminus of the A-fragment first crosses the membrane, whereas the NH2-terminal region follows behind. The possibility of using nontoxic variants of diphtheria toxin as vectors to introduce peptides into the cytosol to elicit MHC class I-restricted immune response and clonal expansion of the relevant CD8+ cytotoxic T lymphocytes is discussed.

摘要

白喉毒素属于一类能够进入动物细胞胞质溶胶的毒性蛋白。我们在此研究了白喉毒素氨基末端延伸对其转运至胞质溶胶能力的影响。通过重组DNA技术,将编码12 - 30个氨基酸的肽段的DNA片段与突变毒素基因的5'端融合。所得DNA构建体在体外进行转录和翻译。翻译产物与细胞结合,然后暴露于低pH值以诱导跨细胞膜转运。在这些条件下,所有测试的寡肽,包括三种病毒肽和白喉毒素的前导肽,都与毒素的酶部分(A片段)一起转运至胞质溶胶。疏水性序列和高电荷序列均未阻断转运。这些结果与一种模型相符,即A片段的羧基末端首先穿过膜,而氨基末端区域随后跟进。讨论了使用白喉毒素无毒变体作为载体将肽段引入胞质溶胶以引发MHC I类限制性免疫反应和相关CD8 + 细胞毒性T淋巴细胞克隆扩增的可能性。

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