Muniz Alberto, Betts Brandi S, Trevino Arnoldo R, Buddavarapu Kalyan, Roman Ricardo, Ma Jian-Xing, Tsin Andrew T C
Department of Biology, The University of Texas at San Antonio, San Antonio, Texas 78249, USA.
Biochemistry. 2009 Jul 28;48(29):6854-63. doi: 10.1021/bi9002937.
In the classic retinoid cycle, 11-cis retinol is synthesized in the retinal pigment epithelium (RPE) by two enzymes: Isomerase I (RPE65) and lecithin:retinol acyltransferase (LRAT). The purpose of this study is to provide experimental evidence for two active isomerases in the cone-dominated chicken eye: an LRAT-dependent Isomerase I in the RPE and an ARAT (acyl CoA:retinol acyltransferase)-dependent isomerase (Isomerase II) in the retina. First, we show that whole chicken retina in vitro, removed from the RPE/choroid and sclera, produces 11-cis retinoids upon light exposure, indicating the existence of RPE-independent isomerase (Isomerase II) activity in the retina. Reverse transcriptase polymerase chain reaction studies show high levels of RPE65 expression in the RPE, low levels in the retina, and none in primary Muller cell cultures, indicating the presence of Isomerase I in the RPE and a minimal amount in the retina. Activities of the RPE and retina isomerases were then measured by enzyme assays with specific enzyme inhibitors. 2,2'-Bipyridine, a known Isomerase I inhibitor, and N-ethylmaleimide (NEM), a known LRAT inhibitor, significantly reduced Isomerase I activity but not Isomerase II activity. Progesterone, a known ARAT inhibitor, completely blocked Isomerase II activity but not Isomerase I activity. Thus, this study reports novel results for distinguishing the biochemical properties of Isomerase I from those of Isomerase II, as well a difference in their locations in the chicken eye. On the basis of these differences, the cone-dominated chicken eye must contain two retinoid cycles: a classic visual cycle for retinoid exchange between the RPE and the retina supported by Isomerase I in the RPE and an additional visual cycle for retinoid processing in the retina supported by Isomerase II.
在经典的视黄醛循环中,11-顺式视黄醇由视网膜色素上皮(RPE)中的两种酶合成:异构酶I(RPE65)和卵磷脂:视黄醇酰基转移酶(LRAT)。本研究的目的是为以视锥细胞为主的鸡眼中的两种活性异构酶提供实验证据:RPE中依赖LRAT的异构酶I和视网膜中依赖酰基辅酶A:视黄醇酰基转移酶(ARAT)的异构酶(异构酶II)。首先,我们表明,从RPE/脉络膜和巩膜分离出来的体外全鸡视网膜在光照下会产生11-顺式视黄醛,这表明视网膜中存在不依赖RPE的异构酶(异构酶II)活性。逆转录聚合酶链反应研究表明,RPE65在RPE中高表达,在视网膜中低表达,在原代穆勒细胞培养物中不表达,这表明异构酶I存在于RPE中,在视网膜中含量极少。然后通过使用特异性酶抑制剂的酶测定法测量RPE和视网膜异构酶的活性。2,2'-联吡啶是一种已知的异构酶I抑制剂,N-乙基马来酰亚胺(NEM)是一种已知的LRAT抑制剂,它们显著降低了异构酶I的活性,但没有降低异构酶II的活性。孕酮是一种已知的ARAT抑制剂,它完全阻断了异构酶II的活性,但没有阻断异构酶I的活性。因此,本研究报告了区分异构酶I和异构酶II生化特性的新结果,以及它们在鸡眼中位置的差异。基于这些差异,以视锥细胞为主的鸡眼必须包含两个视黄醛循环:一个是由RPE中的异构酶I支持的RPE与视网膜之间视黄醛交换的经典视觉循环,另一个是由异构酶II支持的视网膜中视黄醛加工的额外视觉循环。