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新型视网膜上皮膜蛋白REMP的发育表达与分子克隆

Developmental expression and molecular cloning of REMP, a novel retinal epithelial membrane protein.

作者信息

Philp N, Chu P, Pan T C, Zhang R Z, Chu M L, Stark K, Boettiger D, Yoon H, Kieber-Emmons T

机构信息

Pennsylvania College of Optometry, Philadelphia 19141-3399, USA.

出版信息

Exp Cell Res. 1995 Jul;219(1):64-73. doi: 10.1006/excr.1995.1205.

Abstract

The retinal pigment epithelium (RPE), like other transport epithelia, has a polarized distribution of membrane and cytoskeletal proteins. The establishment of a polarized phenotype is an essential step in the differentiation of the RPE and the development and maintenance of visual function. Using a monoclonal antibody (MAb 3C4) we have identified a novel membrane protein that is uniquely expressed in chick RPE. We have referred to this protein as REMP for retinal epithelial membrane protein. In these studies we characterized the expression and distribution of this protein during embryonic development and determined its primary structure by cDNA cloning. The developmental expression of REMP was examined by immunocytochemical localization. REMP was first detected in the chick RPE at Embryonic Day 5 (E5) in both apical and basolateral membranes. By E14 the distribution of REMP was restricted to the basolateral surface of the RPE cells. Biochemical fractionation and surface labeling of RPE cells suggested that REMP was an integral protein. The gene encoding REMP was isolated from an E15 chick RPE cDNA library, cloned into lambda gt11, and screened with MAb 3C4. The cDNA was sequenced and found to contain one 1350-bp open reading frame encoding for a 450-amino-acid protein. The deduced amino-acid sequence of REMP shares 32.9% identity with MCT1, a monocarboxylate transporter (Garcia, Goldstein, Pathak, Anderson, and Brown, Cell, 76, 865-873, 1994). By Northern blot analysis, REMP mRNA was detected only in RPE cells. There was an increase in the expression REMP transcript during development but when RPE cells were grown in primary culture the expression of REMP was turned off. The unique expression of REMP in the RPE in vivo would suggest a role for this protein in development and maintenance of normal retinal function.

摘要

视网膜色素上皮(RPE)与其他转运上皮一样,具有膜蛋白和细胞骨架蛋白的极化分布。极化表型的建立是RPE分化以及视觉功能发育和维持的关键步骤。我们使用单克隆抗体(MAb 3C4)鉴定了一种在鸡RPE中独特表达的新型膜蛋白。我们将这种蛋白称为视网膜上皮膜蛋白(REMP)。在这些研究中,我们表征了该蛋白在胚胎发育过程中的表达和分布,并通过cDNA克隆确定了其一级结构。通过免疫细胞化学定位检测REMP的发育表达。在胚胎第5天(E5),在鸡RPE的顶端和基底外侧膜中首次检测到REMP。到E14时,REMP的分布局限于RPE细胞的基底外侧表面。RPE细胞的生化分级分离和表面标记表明REMP是一种整合蛋白。从E15鸡RPE cDNA文库中分离出编码REMP的基因,克隆到λgt11中,并用MAb 3C4进行筛选。对该cDNA进行测序,发现其包含一个1350bp的开放阅读框,编码一个450个氨基酸的蛋白。REMP推导的氨基酸序列与单羧酸转运蛋白MCT1有32.9%的同一性(Garcia、Goldstein、Pathak、Anderson和Brown,《细胞》,76,865 - 873,1994)。通过Northern印迹分析,仅在RPE细胞中检测到REMP mRNA。在发育过程中REMP转录本的表达增加,但当RPE细胞在原代培养中生长时,REMP的表达被关闭。REMP在体内RPE中的独特表达表明该蛋白在正常视网膜功能的发育和维持中起作用。

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