Brian J E, Moore S A, Faraci F M
Department of Anesthesia, and Internal Medicine and Pharmacology, University of Iowa College of Medicine, Iowa City, USA.
Stroke. 1998 Dec;29(12):2600-6. doi: 10.1161/01.str.29.12.2600.
Cyclooxygenase-2 (COX-2) is an inducible isoform of cyclooxygenase. Several types of brain cells in culture can express COX-2 when treated with lipopolysaccharide (LPS) or some cytokines. LPS produces dilatation of cerebral arterioles in vivo through a mechanism that is partially inhibited by indomethacin. In the present study we examined the hypothesis that LPS causes increased expression of COX-2 in brain as well as COX-2-dependent dilatation of cerebral arterioles.
Cranial windows were implanted in anesthetized rats and used to measure diameter of cerebral arterioles under control conditions and during topical application of various agonists and antagonists. Windows were flushed every 30 minutes for 4 hours with vehicle (artificial cerebrospinal fluid; n=5), LPS (100 ng/mL; n=8), LPS and NS-398 (100 micromol/L; n=8), a selective inhibitor of COX-2, or LPS and dexamethasone (1 micromol/L; n=5), which attenuates expression of COX-2. To examine expression of COX-2 protein in vivo, other animals were injected intracisternally with artificial cerebrospinal fluid (n=3) or LPS (40 ng; n=4). Four hours after injection, the leptomeninges were harvested and analyzed by Western blot for expression of COX-2 protein. In a third group of experiments, COX-2 expression and prostaglandin E2 (PGE2) production were determined in leptomeningeal tissue treated for 4 hours ex vivo with vehicle (n=4), LPS (100 ng/mL; n=4), LPS and NS-398 (100 micromol/L; n=4), or LPS and dexamethasone (1 micromol/L; n=4).
LPS caused marked, progressive dilatation of cerebral arterioles, with a maximum increase in diameter of 55+/-9% (mean+/-SEM) at 4 hours. Coapplication of either NS-398 or dexamethasone with LPS reduced dilatation of cerebral arterioles at hours 2 through 4 (P<0.05). In contrast, NS-398 did not inhibit dilatation of cerebral arterioles in response to bradykinin or ADP. In animals injected intracisternally with vehicle, COX-2 protein was expressed at a very low level in leptomeningeal tissue. Intracisternal injection of LPS increased COX-2 protein expression by approximately 20-fold (P<0.05). In leptomeningeal tissue treated ex vivo with LPS, there was also expression of COX-2. Both dexamethasone and NS-398 markedly reduced COX-2 protein expression in ex vivo LPS-treated tissue. PGE2 production was detectable under control conditions in leptomeningeal tissue incubated in vehicle ex vivo for 4 hours (6.5+/-1.1 pmol/mg protein). LPS treatment significantly increased PGE2 production to 12.8+/-1.1 pmol/mg protein (P<0.05). Both dexamethasone and NS-398 significantly attenuated LPS-induced PGE2 production (P<0.05).
LPS increased expression of COX-2 protein in leptomeningeal tissue and caused COX-2-dependent dilatation of cerebral arterioles in vivo. Ex vivo, both NS-398 and dexamethasone suppressed LPS-induced PGE2 production and COX-2 expression in leptomeningeal tissue. Inhibition of LPS-induced dilatation of cerebral arterioles in vivo by NS-398 and dexamethasone suggests that the dilatation was dependent on expression and activity of COX-2. These findings support the concept that exposure of brain to LPS causes cerebral vasodilatation that is dependent in part on expression and activity of COX-2.
环氧化酶 -2(COX -2)是环氧化酶的一种可诱导同工型。培养中的几种类型脑细胞在用脂多糖(LPS)或某些细胞因子处理时可表达COX -2。LPS在体内通过一种可被吲哚美辛部分抑制的机制使脑动脉扩张。在本研究中,我们检验了LPS导致脑内COX -2表达增加以及COX -2依赖性脑动脉扩张这一假说。
在麻醉大鼠中植入颅窗,用于在对照条件下以及局部应用各种激动剂和拮抗剂期间测量脑动脉直径。每隔30分钟用赋形剂(人工脑脊液;n = 5)、LPS(100 ng/mL;n = 8)、LPS与NS -398(100 μmol/L;n = 8,一种COX -2选择性抑制剂)或LPS与地塞米松(1 μmol/L;n = 5,可减弱COX -2表达)冲洗颅窗4小时。为了检测体内COX -2蛋白的表达,向其他动物脑池内注射人工脑脊液(n = 3)或LPS(40 ng;n = 4)。注射后4小时,收集软脑膜并通过蛋白质印迹法分析COX -2蛋白的表达。在第三组实验中,测定用赋形剂(n = 4)、LPS(100 ng/mL;n = 4)、LPS与NS -398(100 μmol/L;n = 4)或LPS与地塞米松(1 μmol/L;n = 4)离体处理4小时的软脑膜组织中的COX -2表达和前列腺素E2(PGE2)产生。
LPS导致脑动脉明显、渐进性扩张,4小时时直径最大增加55±9%(平均值±标准误)。NS -398或地塞米松与LPS共同应用在第2至4小时减少了脑动脉扩张(P < 0.05)。相比之下,NS -398不抑制脑动脉对缓激肽或ADP的扩张反应。在脑池内注射赋形剂的动物中,软脑膜组织中COX -2蛋白以非常低的水平表达。脑池内注射LPS使COX -2蛋白表达增加约20倍(P < 0.05)。在离体用LPS处理的软脑膜组织中也有COX -2表达。地塞米松和NS -398均显著降低离体LPS处理组织中的COX -2蛋白表达。在对照条件下,离体用赋形剂孵育4小时的软脑膜组织中可检测到PGE2产生(6.5±1.1 pmol/mg蛋白)。LPS处理显著增加PGE2产生至12.8±1.1 pmol/mg蛋白(P < 0.05)。地塞米松和NS -398均显著减弱LPS诱导的PGE2产生(P < 0.05)。
LPS增加软脑膜组织中COX -2蛋白的表达,并在体内引起COX -2依赖性脑动脉扩张行为。在离体实验中,NS -398和地塞米松均抑制LPS诱导的软脑膜组织中PGE2产生和COX -2表达。NS -398和地塞米松在体内对LPS诱导的脑动脉扩张的抑制表明这种扩张依赖于COX -2的表达和活性。这些发现支持了脑暴露于LPS会导致部分依赖于COX -2表达和活性的脑血管扩张这一概念。
