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寻找抑制可溶性N-乙基马来酰亚胺敏感因子附着受体介导的膜融合的合成肽。

A search for synthetic peptides that inhibit soluble N-ethylmaleimide sensitive-factor attachment receptor-mediated membrane fusion.

作者信息

Jung Chang H, Yang Yoo-Soo, Kim Jun-Seob, Shin Jae-Il, Jin Yong-Su, Shin Jae Y, Lee Jong H, Chung Koo M, Hwang Jae S, Oh Jung M, Shin Yeon-Kyun, Kweon Dae-Hyuk

机构信息

School of Biotechnology and Bioengineering, Sungkyunkwan University, Gyeonggi-do, Korea.

出版信息

FEBS J. 2008 Jun;275(12):3051-63. doi: 10.1111/j.1742-4658.2008.06458.x. Epub 2008 May 6.

DOI:10.1111/j.1742-4658.2008.06458.x
PMID:18459979
Abstract

Soluble N-ethylmaleimide sensitive-factor attachment receptor (SNARE) proteins have crucial roles in driving exocytic membrane fusion. Molecular recognition between vesicle-associated (v)-SNARE and target membrane (t)-SNARE leads to the formation of a four-helix bundle, which facilitates the merging of two apposing membranes. Synthetic peptides patterned after the SNARE motifs are predicted to block SNARE complex formation by competing with the parental SNAREs, inhibiting neuronal exocytosis. As an initial attempt to identify the peptide sequences that block SNARE assembly and membrane fusion, we created thirteen 17-residue synthetic peptides derived from the SNARE motifs of v- and t-SNAREs. The effects of these peptides on SNARE-mediated membrane fusion were investigated using an in vitro lipid-mixing assay, in vivo neurotransmitter release and SNARE complex formation assays in PC12 cells. Peptides derived from the N-terminal region of SNARE motifs had significant inhibitory effects on neuroexocytosis, whereas middle- and C-terminal-mimicking peptides did not exhibit much inhibitory function. N-terminal mimicking peptides blocked N-terminal zippering of SNAREs, a rate-limiting step in SNARE-driven membrane fusion. Therefore, the results suggest that the N-terminal regions of SNARE motifs are excellent targets for the development of drugs to block SNARE-mediated membrane fusion and neurotransmitter release.

摘要

可溶性N - 乙基马来酰亚胺敏感因子附着受体(SNARE)蛋白在驱动胞吐性膜融合中起关键作用。囊泡相关(v)-SNARE与靶膜(t)-SNARE之间的分子识别导致四螺旋束的形成,这促进了两个相对膜的融合。预测以SNARE基序为模板的合成肽通过与亲本SNARE竞争来阻断SNARE复合物的形成,从而抑制神经元胞吐作用。作为鉴定阻断SNARE组装和膜融合的肽序列的初步尝试,我们从v - 和t - SNARE的SNARE基序中创建了13种17个残基的合成肽。使用体外脂质混合试验、体内神经递质释放以及PC12细胞中的SNARE复合物形成试验研究了这些肽对SNARE介导的膜融合的影响。源自SNARE基序N端区域的肽对神经胞吐作用具有显著抑制作用,而中间和C端模拟肽则没有表现出太多抑制功能。N端模拟肽阻断了SNARE的N端拉链形成,这是SNARE驱动膜融合中的限速步骤。因此,结果表明SNARE基序的N端区域是开发阻断SNARE介导的膜融合和神经递质释放药物的理想靶点。

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