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基质金属蛋白酶组织抑制剂(TIMPs)-1和-3平衡的改变可能会促进圆锥角膜中角膜细胞的凋亡。

Changes in the balance of the tissue inhibitor of matrix metalloproteinases (TIMPs)-1 and -3 may promote keratocyte apoptosis in keratoconus.

作者信息

Matthews Fiona J, Cook Stuart D, Majid Mohammed A, Dick Andrew D, Smith Valerie A

机构信息

University of Bristol, Academic Unit of Ophthalmology, Bristol Eye Hospital, Lower Maudlin Street, Bristol, BS1 2LX, UK.

出版信息

Exp Eye Res. 2007 Jun;84(6):1125-34. doi: 10.1016/j.exer.2007.02.013. Epub 2007 Mar 7.

DOI:10.1016/j.exer.2007.02.013
PMID:17449031
Abstract

Keratoconus is a disease in which the central cornea becomes thinned. This could result from corneal stromal cell apoptosis or be induced or perpetuated by the activation of matrix degrading enzymes, particularly members of the matrix metalloproteinase (MMP) family. In some circumstances, the MMP inhibitors TIMP-1 and TIMP-3 exhibit anti-apoptotic and pro-apoptotic properties, respectively. Because they potentially influence keratoconus progression, the effects of TIMP-1 and TIMP-3 on stromal cell viability were investigated. The TIMP-1 and TIMP-3 proteins were over-expressed in cultured corneal stromal cells by using the adenoviral vectors RAdTIMP-1 and RAdTIMP-3 and quantified by enzyme-linked immunosorbant assay (ELISA). Apoptotic cells were detected by TUNEL and caspase-3 activity. The anti-apoptotic effects of TIMP-1 were investigated by co-infecting it with RAdTIMP-1 and RAdTIMP-3 and by adding TIMP-1 protein to stromal cell cultures prior to infecting them with RAdTIMP-3. Immunohistochemistry was used to localise and determine relative numbers of apoptotic and TIMP producing stromal cells in sections of normal and keratoconic corneas. The results showed that over-expression of TIMP-3 induced apoptosis in corneal stromal cell cultures. Up-regulated TIMP-1 production or the addition of exogenous TIMP-1 protein prevented stromal cell overgrowth, changed stromal cell morphology and reduced the extent of TIMP-3 induced apoptosis. Localised relative concentrations of TIMP-1/TIMP-3 could thus determine whether these cells remain viable or become apoptotic. This may be relevant to the keratoconic condition since significantly more apoptotic cells were identified in the anterior stroma of keratoconic corneas than normal corneas and the majority of theTIMP-1 and TIMP-3 producing stromal cells were also located in this region.

摘要

圆锥角膜是一种中央角膜变薄的疾病。这可能是由角膜基质细胞凋亡引起的,或者是由基质降解酶的激活所诱导或持续存在的,尤其是基质金属蛋白酶(MMP)家族的成员。在某些情况下,MMP抑制剂TIMP-1和TIMP-3分别表现出抗凋亡和促凋亡特性。由于它们可能影响圆锥角膜的进展,因此研究了TIMP-1和TIMP-3对基质细胞活力的影响。通过使用腺病毒载体RAdTIMP-1和RAdTIMP-3在培养的角膜基质细胞中过表达TIMP-1和TIMP-3蛋白,并通过酶联免疫吸附测定(ELISA)进行定量。通过TUNEL和caspase-3活性检测凋亡细胞。通过将TIMP-1与RAdTIMP-1和RAdTIMP-3共感染,并在将基质细胞培养物用RAdTIMP-3感染之前向其中添加TIMP-1蛋白,研究了TIMP-1的抗凋亡作用。免疫组织化学用于定位和确定正常角膜和圆锥角膜切片中凋亡和产生TIMP的基质细胞的相对数量。结果表明,TIMP-3的过表达诱导了角膜基质细胞培养物中的细胞凋亡。TIMP-1产生的上调或外源性TIMP-1蛋白的添加可防止基质细胞过度生长,改变基质细胞形态并减少TIMP-3诱导的细胞凋亡程度。因此,TIMP-1/TIMP-3的局部相对浓度可以决定这些细胞是保持存活还是发生凋亡。这可能与圆锥角膜的病情相关,因为在圆锥角膜的前基质中发现的凋亡细胞明显多于正常角膜,并且大多数产生TIMP-1和TIMP-3的基质细胞也位于该区域。

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