Li De-Quan, Chen Zhuo, Song Xiu Jun, Luo Lihui, Pflugfelder Stephen C
Ocular Surface Center, Cullen Eye Institute, Department of Ophthalmology, Baylor College of Medicine, 6565 Fannin Street, Houston, TX 77030, USA.
Invest Ophthalmol Vis Sci. 2004 Dec;45(12):4302-11. doi: 10.1167/iovs.04-0299.
To investigate whether exposure of human corneal epithelial cells to hyperosmotic stress activates the c-Jun NH(2)-terminal kinase (JNK) stress-activated protein kinase (SAPK) pathway, and stimulates production of the matrix metalloproteinases (MMPs): gelatinase (MMP-9), collagenases (MMP-1 and -13), and stromelysin (MMP-3).
Primary human corneal epithelial cells cultured in normal osmolar medium (312 mOsM) were exposed to media with higher osmolarity (350-500 mOsM) achieved by adding NaCl, with or without SB202190, an inhibitor of the JNK pathway; dexamethasone; or doxycycline for different lengths of time. The conditioned media were collected after 24 hours of exposure for zymography and ELISA. Total RNA was extracted from cultures treated for 6 hours and subjected to semiquantitative RT-PCR. Cells treated for 5 to 60 minutes were lysed in RIPA buffer and subjected to Western blot with phospho (p)-specific antibodies against p-JNK and p-c-Jun. JNK1 activation was also detected with an immunoassay system.
The concentrations of MMP-9, -1, and -3 proteins in 24-hour conditioned media of corneal epithelial cells progressively increased as the media's osmolarity was increased from 312 to 500 mOsM by the addition of NaCl. The concentration of MMP-13 progressively increased to a peak at 450 mOsM. Active p-JNK-1, p-JNK-2, and p-c-Jun were detected by Western blot as early as 5 minutes and peaked at 60 minutes in cells exposed to hyperosmolar media. The levels of p-JNK-1, p-JNK-2, and p-c-Jun correlated positively with the osmolarity of the culture media. The p-JNK inhibitor SB202190 and doxycycline markedly inhibited the stimulation of p-JNK-1, p-JNK-2, and p-c-Jun, as well as MMP-9, -1, -13, and -3 at both the mRNA and protein levels in the cells exposed to hyperosmolar media.
Expression and production of MMP-9, -1, -13, and -3 by human corneal epithelial cells correlated positively with increasing media osmolarity. This increase was mediated at least in part through activation of the JNK SAPK pathway. Doxycycline, an agent used to treat MMP-mediated ocular surface disease, inhibited the hyperosmolarity-induced MMP production and JNK activation. The relevance of these findings to stimulated production of MMPs by the elevated tear osmolarity in dry eye remains to be determined.
研究人角膜上皮细胞暴露于高渗应激时是否会激活c-Jun氨基末端激酶(JNK)应激激活蛋白激酶(SAPK)通路,并刺激基质金属蛋白酶(MMP)的产生,即明胶酶(MMP-9)、胶原酶(MMP-1和-13)以及基质溶解素(MMP-3)。
将在正常渗透压培养基(312 mOsM)中培养的原代人角膜上皮细胞暴露于通过添加氯化钠实现更高渗透压(350 - 500 mOsM)的培养基中,添加或不添加JNK通路抑制剂SB202190、地塞米松或强力霉素,作用不同时长。暴露培养24小时后收集条件培养基用于酶谱分析和酶联免疫吸附测定(ELISA)。从处理6小时的培养物中提取总RNA并进行半定量逆转录聚合酶链反应(RT-PCR)。将处理5至60分钟的细胞在放射免疫沉淀分析(RIPA)缓冲液中裂解,并用针对磷酸化(p)-JNK和p-c-Jun的特异性抗体进行蛋白质免疫印迹分析。还使用免疫测定系统检测JNK1的激活情况。
通过添加氯化钠将角膜上皮细胞24小时条件培养基中的渗透压从312 mOsM提高到500 mOsM时,MMP-9、-1和-3蛋白的浓度逐渐增加。MMP-13的浓度在450 mOsM时逐渐增加至峰值。在暴露于高渗培养基的细胞中,通过蛋白质免疫印迹分析最早在5分钟时检测到活性p-JNK-1、p-JNK-2和p-c-Jun,60分钟时达到峰值。p-JNK-1、p-JNK-2和p-c-Jun的水平与培养基的渗透压呈正相关。p-JNK抑制剂SB202190和强力霉素在mRNA和蛋白质水平上均显著抑制了暴露于高渗培养基的细胞中p-JNK-1、p-JNK-2和p-c-Jun以及MMP-9、-1、-13和-3的刺激。
人角膜上皮细胞中MMP-9、-1、-13和-3的表达及产生与培养基渗透压升高呈正相关。这种增加至少部分是通过JNK SAPK通路的激活介导的。强力霉素是一种用于治疗MMP介导的眼表疾病的药物,它抑制了高渗诱导的MMP产生和JNK激活。这些发现与干眼时泪液渗透压升高刺激MMP产生的相关性仍有待确定。
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