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视网膜细胞结构和光感受器结构维持中蛋白质异戊二烯化的体内需求。

In vivo requirement of protein prenylation for maintenance of retinal cytoarchitecture and photoreceptor structure.

作者信息

Pittler S J, Fliesler S J, Fisher P L, Keller P K, Rapp L M

机构信息

Department of Biochemistry and Molecular Biology, College of Medicine, University of South Alabama, Mobile 36688-0002, USA.

出版信息

J Cell Biol. 1995 Jul;130(2):431-9. doi: 10.1083/jcb.130.2.431.

Abstract

Recent studies have demonstrated that inhibition of mevalonate synthesis in cultured cells leads to altered cell morphology due to inhibition of protein prenylation. To investigate the effects in vivo of mevalonate deprivation in nondividing, terminally differentiated neural cells, we have analyzed the effects on retinal tissue of intravitreal injection of lovastatin, a potent inhibitor of the mevalonate-producing enzyme, HMG-CoA reductase. A single injection of lovastatin (0.25 mumol) produced profound dysplastic-like changes in adult rat retinas primarily involving the photoreceptor layer. Within 2 d after injection, photoreceptor nuclei migrated in a circular pattern resulting in the formation of rosette-like structures by 4 d. Also during this period, photoreceptor inner and outer segment degeneration was evident. By 21 d, intact photoreceptor nuclei with remnants of inner and outer segments were dispersed throughout all retinal layers. To investigate the biochemical specificity of the lovastatin-induced alterations, and to distinguish the relative importance of the various branches of the mevalonate pathway, the incorporation of [3H]acetate into retinal lipids was examined in the presence and absence of metabolic inhibitors. HPLC analysis of lovastatin-treated retinas revealed a dramatic reduction in the incorporation of intravitreally injected [3H]acetate into nonsaponifiable lipids, compared with controls. In contrast, intravitreal injection of NB-598, a specific inhibitor of squalene epoxidase, eliminated the conversion of newly synthesized squalene to sterols without obvious pathology. Hence, involvement to the sterol branch of isoprenoid metabolism in the lovastatin-induced morphologic disruption was obviated. Intravitreal injection of 0.27 mumol of N-acetyl-S-trans,trans-farnesyl-L-cysteine (AFC), an inhibitor of carboxyl methyltransferase activity and prenylated protein function, produced morphologic changes that were virtually indistinguishable from those induced with lovastatin. These results implicate a defect in protein prenylation in the lovastatin-induced retinal degeneration, and suggest the presence of a dynamic pathway in the retina that requires isoprenylated proteins to maintain retinal cytoarchitecture.

摘要

最近的研究表明,在培养细胞中抑制甲羟戊酸合成会由于抑制蛋白质异戊二烯化而导致细胞形态改变。为了研究在非分裂、终末分化的神经细胞中甲羟戊酸缺乏在体内的影响,我们分析了玻璃体内注射洛伐他汀(一种甲羟戊酸生成酶HMG-CoA还原酶的有效抑制剂)对视网膜组织的影响。单次注射洛伐他汀(0.25 μmol)在成年大鼠视网膜中产生了严重的发育异常样变化,主要累及光感受器层。注射后2天内,光感受器细胞核呈圆形迁移,到4天时形成玫瑰花结样结构。同样在此期间,光感受器内、外段退化明显。到21天时,带有内、外段残余的完整光感受器细胞核分散在所有视网膜层中。为了研究洛伐他汀诱导的改变的生化特异性,并区分甲羟戊酸途径各分支的相对重要性,在存在和不存在代谢抑制剂的情况下检测了[3H]乙酸掺入视网膜脂质的情况。与对照组相比,对洛伐他汀处理的视网膜进行HPLC分析显示,玻璃体内注射的[3H]乙酸掺入非皂化脂质的量显著减少。相反,玻璃体内注射角鲨烯环氧化酶的特异性抑制剂NB-598消除了新合成的角鲨烯向固醇的转化,且无明显病理变化。因此,排除了类异戊二烯代谢的固醇分支参与洛伐他汀诱导的形态破坏。玻璃体内注射0.27 μmol N-乙酰-S-反,反-法尼基-L-半胱氨酸(AFC),一种羧基甲基转移酶活性和异戊二烯化蛋白功能的抑制剂,产生的形态变化与洛伐他汀诱导的变化几乎无法区分。这些结果表明蛋白质异戊二烯化缺陷与洛伐他汀诱导的视网膜变性有关,并提示视网膜中存在一条动态途径,该途径需要异戊二烯化蛋白来维持视网膜细胞结构。

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