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视网膜视杆细胞外段膜与模型膜之间的融合:光感受器外周蛋白/视网膜变性慢病毒的作用。

Fusion between retinal rod outer segment membranes and model membranes: a role for photoreceptor peripherin/rds.

作者信息

Boesze-Battaglia K, Lamba O P, Napoli A A, Sinha S, Guo Y

机构信息

Department of Molecular Biology, University of Medicine and Dentistry of New Jersey-SOM, Stratford 08084, USA.

出版信息

Biochemistry. 1998 Jun 30;37(26):9477-87. doi: 10.1021/bi980173p.

DOI:10.1021/bi980173p
PMID:9649331
Abstract

Peripherin/rds plays an essential role in the maintenance of photoreceptor rod cell disk membrane structure. The purification of this protein to homogeneity [Boesze-Battaglia, K., et al. (1997) Biochemistry 36, 6835-6846] has allowed us to characterize the functional role of peripherin/rds in the maintenance of rod outer segment (ROS) membrane fusion processes. Utilizing a cell-free fusion assay system, we report that the fusion of R18-labeled ROS plasma membrane (R18-PM) with disk membranes or peripherin/rds-enriched large unilammellar vesicles (LUVs) is inhibited upon trypsinolysis of peripherin/rds. To understand this phenomenon, we tested the ability of a series of overlapping synthetic C-terminal peripherin/rds peptides to mediate model membrane fusion. Within the 63 amino acid long region of the C-terminus, we identified a minimal 15 residue long amino acid sequence (PP-5), which is necessary to promote membrane fusion. PP-5 was able to inhibit R18-PM disk membrane fusion and promoted ANTS/DPX contents mixing in a pure vesicle system. This peptide (PP-5) promoted calcium-induced vesicle aggregation of phosphatidylethanolamine:phosphatidylserine LUVs. FTIR analysis confirmed the structural prediction of this peptide as alpha-helical. When modeled as an alpha-helix, this peptide is amphiphilic with a hydrophobicity index of 0.75 and a hydrophobic moment of 0.59. PP-5 has substantial biochemical and functional homology with other well-characterized membrane fusion proteins. These results demonstrate the necessity for peripherin/rds in ROS membrane fusion, specifically the requirement for an intact C-terminal region of this protein.

摘要

外周蛋白/视网膜变性慢(Peripherin/rds)在光感受器视杆细胞盘膜结构的维持中起着至关重要的作用。该蛋白纯化至同质状态[Boesze - Battaglia, K., 等人(1997年)《生物化学》36卷,6835 - 6846页]使我们能够表征外周蛋白/视网膜变性慢在视杆外段(ROS)膜融合过程维持中的功能作用。利用无细胞融合检测系统,我们报告称,在用胰蛋白酶消化外周蛋白/视网膜变性慢后,R18标记的ROS质膜(R18 - PM)与盘膜或富含外周蛋白/视网膜变性慢的大单层囊泡(LUVs)的融合受到抑制。为理解这一现象,我们测试了一系列重叠的合成C端外周蛋白/视网膜变性慢肽介导模型膜融合的能力。在C端63个氨基酸长的区域内,我们鉴定出一个最小的15个残基长的氨基酸序列(PP - 5),它是促进膜融合所必需的。PP - 5能够抑制R18 - PM盘膜融合,并在纯囊泡系统中促进ANTS/DPX含量混合。该肽(PP - 5)促进了钙诱导的磷脂酰乙醇胺:磷脂酰丝氨酸LUVs的囊泡聚集。傅里叶变换红外光谱(FTIR)分析证实了该肽的α - 螺旋结构预测。当建模为α - 螺旋时,该肽具有两亲性,疏水指数为0.75,疏水矩为0.59。PP - 5与其他已充分表征的膜融合蛋白具有显著的生化和功能同源性。这些结果证明了外周蛋白/视网膜变性慢在ROS膜融合中的必要性,特别是该蛋白完整C端区域的必要性。

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