Zenkel Matthias, Pöschl Ernst, von der Mark Klaus, Hofmann-Rummelt Carmen, Naumann Gottfried O H, Kruse Friedrich E, Schlötzer-Schrehardt Ursula
Department of Ophthalmology, University of Erlangen-Nürnberg, Germany.
Invest Ophthalmol Vis Sci. 2005 Oct;46(10):3742-52. doi: 10.1167/iovs.05-0249.
To identify and characterize genes differentially expressed in anterior segment tissues of eyes with pseudoexfoliation (PEX) syndrome and glaucoma.
Anterior segment tissues (iris, ciliary processes, lens epithelium) were obtained from eight surgically enucleated eyes with PEX-associated open-angle or closed-angle glaucomas and eight age-matched glaucomatous control eyes without PEX. cDNA libraries were generated from three PEX and three control specimens, and their gene expression patterns were compared by means of cDNA subtraction. Differentially expressed clones from the subtracted cDNA libraries were sequenced, and their differential expression was verified by means of RT-PCR, virtual Northern blot analysis, and in situ hybridization with specific RNA probes.
Subtraction of cDNA libraries identified 27 candidate genes for differential expression in PEX tissues, of which 23 genes were confirmed by virtual Northern blot, RT-PCR, and in situ hybridization. One set of genes consistently upregulated in anterior segment tissues from different patients with PEX comprised latent transforming growth factor binding proteins (LTBP-1 and -2), which are structural components of elastic microfibrils, the cross-linking enzyme transglutaminase-2 (TGase-2), tissue inhibitor of matrix metalloproteinase-2 (TIMP-2), A-kinase anchor protein-2 (AKAP-2), apolipoprotein D, and the adenosine receptor-A3 (AdoR-A3). Genes reproducibly downregulated in PEX tissues included TIMP-1, clusterin, microsomal glutathione-S-transferase-1 (mGST-1), and serum amyloid A1. Further transcripts, such as elastase, GST-T1, integrin beta4, and dehydrocholesterol reductase, did not show a consistent differential expression pattern in tissues obtained from different patients. Although fibrillin-1 was not isolated from subtracted cDNA libraries, upregulated expression of this elastic microfibrillar component was also demonstrated by RT-PCR and in situ hybridization.
Differentially expressed genes with a high level of reproducibility in different tissues and different patients with PEX syndrome are mainly related to extracellular matrix metabolism and cellular stress. The underlying pathophysiology of PEX syndrome appears to be associated with an excessive production of elastic microfibril components, enzymatic cross-linking processes, a proteolytic imbalance between matrix metalloproteinases and their inhibitors, and increased cellular and oxidative stress supporting the notion of PEX syndrome as a stress-induced elastic microfibrillopathy.
鉴定并表征在假性剥脱(PEX)综合征和青光眼患者眼前节组织中差异表达的基因。
从8只因手术摘除的患有PEX相关开角型或闭角型青光眼的眼睛以及8只年龄匹配的无PEX的青光眼对照眼中获取眼前节组织(虹膜、睫状体、晶状体上皮)。从3个PEX样本和3个对照样本中构建cDNA文库,并通过cDNA消减技术比较它们的基因表达模式。对消减后的cDNA文库中差异表达的克隆进行测序,并通过RT-PCR、虚拟Northern印迹分析以及用特异性RNA探针进行原位杂交来验证它们的差异表达。
cDNA文库消减鉴定出27个在PEX组织中差异表达的候选基因,其中23个基因通过虚拟Northern印迹、RT-PCR和原位杂交得到证实。一组在不同PEX患者眼前节组织中持续上调表达的基因包括潜伏转化生长因子结合蛋白(LTBP-1和-2),它们是弹性微原纤维的结构成分、交联酶转谷氨酰胺酶-2(TGase-2)、基质金属蛋白酶-2组织抑制剂(TIMP-2)、A激酶锚定蛋白-2(AKAP-2)、载脂蛋白D和腺苷受体-A3(AdoR-A3)。在PEX组织中可重复性下调的基因包括TIMP-1、簇集蛋白、微粒体谷胱甘肽-S-转移酶-1(mGST-1)和血清淀粉样蛋白A1。其他转录本,如弹性蛋白酶、GST-T1、整合素β4和脱氢胆固醇还原酶,在不同患者获得的组织中未显示出一致的差异表达模式。虽然原纤维蛋白-1未从消减后的cDNA文库中分离出来,但通过RT-PCR和原位杂交也证实了这种弹性微原纤维成分的上调表达。
在不同组织和不同PEX综合征患者中具有高度可重复性的差异表达基因主要与细胞外基质代谢和细胞应激有关。PEX综合征潜在的病理生理学似乎与弹性微原纤维成分的过度产生、酶促交联过程、基质金属蛋白酶与其抑制剂之间的蛋白水解失衡以及细胞和氧化应激增加有关,这支持了PEX综合征是一种应激诱导的弹性微原纤维病的观点。
