Ischemic preconditioning and lipopolysaccharide attenuate nuclear factor-kappaB activation and gene expression of inflammatory cytokines in the ischemia-reperfused rat heart.

G. Hiasa, M. Hamada, Shuntaro Ikeda, Kunio Hiwada
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引用次数: 52

Abstract

Ischemic preconditioning (IP) and pretreatment with lipopolysaccharide (LPS) reduce myocardial infarct size, but the precise mechanisms remain unknown. Rats were divided into 3 groups: the Control (C) group was subjected to 30 min ischemia followed by 3 h reperfusion; the IP and LPS groups had the same ischemia-reperfusion (I-R) insult with either preconditioning stimuli or pretreatment with LPS, respectively. Infarct size was smaller in the IP (23.4+/-2.3% of risk zone size) and LPS groups (28.5+/-2.0% of risk zone size) than in the C group (52.3+/-3.4% of risk zone size). Nuclear factor kappa-B (NF-kappaB) binding activity increased at 30 min reperfusion and declined thereafter, then rose again at 3 h reperfusion in the C group. The values in the IP (362% of control) and LPS (324% of control) groups were higher before I-R, and then decreased from 30 min (46% and 64% of control, respectively) until 3 h reperfusion (22% and 36% of control, respectively). Nuclear staining of NF-kappaB after reperfusion was less in the IP and LPS groups than in the C group. Expressions of cytokine mRNAs (interleukin-1beta, interleukin-6 and tumor necrosis factor-alpha) were detected 30 min after the onset of reperfusion and their levels remained high after 3 h of reperfusion. These expressions of cytokine mRNAs after I-R were substantially suppressed by IP and LPS, although IP and LPS alone induced modest expressions of these cytokine mRNAs. These data suggest that IP and LPS contribute to infarct size reduction via the downregulation of NF-kappaB and the attenuation of cytokine gene expression.
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缺血预处理和脂多糖可减弱缺血再灌注大鼠心脏核因子κ b的活化和炎症因子的基因表达。
缺血预处理(IP)和脂多糖(LPS)预处理可减少心肌梗死面积,但其确切机制尚不清楚。将大鼠分为3组:对照组(C)缺血30min,再灌注3h;预处理刺激和LPS预处理组缺血再灌注损伤程度相同。梗死面积在IP组(23.4+/-2.3%的危险区大小)和LPS组(28.5+/-2.0%的危险区大小)小于C组(52.3+/-3.4%的危险区大小)。C组核因子κ b (nf - κ b)结合活性在再灌注30min时升高,再灌注30min后下降,再灌注3h时再次升高。IP组(对照组的362%)和LPS组(对照组的324%)在I-R前数值较高,然后在再灌注30 min(分别占对照组的46%和64%)至3 h(分别占对照组的22%和36%)数值下降。再灌注后,IP组和LPS组NF-kappaB核染色明显少于C组。细胞因子mrna(白细胞介素-1 β、白细胞介素-6和肿瘤坏死因子α)在再灌注30min后表达,在再灌注3h后仍保持较高水平。这些细胞因子mrna在I-R后的表达被IP和LPS显著抑制,尽管IP和LPS单独诱导了这些细胞因子mrna的适度表达。这些数据表明,IP和LPS通过下调NF-kappaB和细胞因子基因表达的衰减来减少梗死面积。
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