The Role of Toll-Like Receptors and Nuclear Factor κB p65 Protein in the Pathogenesis of Otitis Media

The role of Toll-like receptor 4 (TLR4) and nuclear factor κB p65 (NF-κB p65) proteins in the pathogenesis of otitis media is explored. In recent years, the incidence of otitis media has been rising globally, becoming a significant threat to human health. More and more studies have found that Toll-like receptor 4 (TLR4), as a member of the Toll-like receptor family, can promote the generation of inflammatory factors and is closely related to the body’s immune response and inflammatory response. Nuclear factor-κB p65 (NF-κB p65) is a nuclear transcription factor that can interact with various cytokines, growth factors, and apoptotic factors, participating in processes such as oxidative stress, apoptosis, and inflammation in the body [1]. This article elaborates on the structure, function, and signaling pathways of TLR4 and NF-κB p65 proteins in the pathogenesis of otitis media, aiming to provide more precise targets and better therapeutic efficacy for the diagnosis and treatment of otitis media. The role of inflammation in disease.

Role of nuclear factor kappa B in central nervous system regeneration

Activation of nuclear factor kappa B （NF-κB） is a hallmark of various central nervous system （CNS） pathologies. Neuron-specific inhibition of its transcriptional activator subunit RelA, also referred to as p65, promotes neuronal survival under a range of conditions, i.e., for ischemic or excitotoxic insults. In macro- and microglial cells, post-lesional activation of NF-κB triggers a growth-permissive program which contributes to neural tissue inflammation, scar formation, and the expression of axonal growth inhibitors. Intriguingly, inhibition of such inducible NF-~B in the neuro-glial compartment, i.e., by genetic ablation of RelA or overexpression of a trans- dominant negative mutant of its upstream regulator IκBa, significantly enhances functional recovery and promotes axonal regeneration in the mature CNS. By contrast, depletion of the NF-κB subunit p50, which lacks transcriptional activator function and acts as a transcriptional repressor on its own, causes precocious neuronal loss and exacerbates axonal degeneration in the lesioned brain. Collectively, the data imply that NF-κB orchestrates a multicellular pro- gram in which κB-dependent gene expression establishes a growth-repulsive terrain within the post-lesioned brain that limits structural regeneration of neuronal circuits. Considering these subunit-specific functions, interference with the NF-κB pathway might hold clinical potentials to improve functional restoration following traumatic CNS injury.

Inhibition of p38 mitogen-activated protein kinase attenuates experimental autoimmune hepatitis: Involvement of nuclear factor kappa B

To investigate the role of p38 mitogen-activated protein kinase （p38MAPK） in murine experimental autoimmune hepatitis （EAH）.METHODS： To induce EAH, the syngeneic S-100 antigen emulsified in complete Freud＇s adjuvant was injected intraperitoneally into adult male C57BI/6 mice. Liver injury was assessed by serum ALT and liver histology. The expression and activity of p38 MAPK were measured by Western blot and kinase activity assays. In addition, DNA binding activities of nuclear factor kappa B （NF-KB） were analyzed by electrophoretic mobility shift assay. The effects of SB203580, a specific p38 MAPK inhibitor, on liver injuries and expression of proinflammatory cytokines （interferon-y, IL-12, IL-1β and TNF-α） were observed.RESULTS： The activity of p38 MAPK and NF-~：B was increased and reached its peak 14 or 21 d after the first syngeneic S-100 administration. Inhibition of p38 MAPK activation by SB203580 decreased the activation of NF-~：B and the expression of proinflammatory cytokines. Moreover, hepatic injuries were improved significantly after SB203580 administration.

Isoflavone Attenuates the Nuclear Transcription Factor Kappa B (NF-<i>κ</i>B) Activation on MPP⁺-Induced Apoptosis of PC12 Cells

Objective: To explore the underlying molecular mechanisms of cellular response to the challenge by 1-methyl-4-phenylpyridinium (MPP+)-induced apoptosis of PC12 cells, an in vitro cell model for Parkinson’s disease, and the effect of NF-κB activation on the protection of Parkinson’s disease by Isoflavone (I). Methods: PC12 cells were used to establish the cell model of Parkinson’s disease, and are divided into five groups: control group;MPP+ group;I (Isoflavone) + MPP+ group;I group;SN-50 + MPP+ group. The content of NF-κB in PC12 cells was determined by immunocytochemistry;The viability of PC12 cells after treated with cell-permeable NF-κB inhibitor SN-50 and cell viability were measured by MTT assay;the expression levels of NF-κB p65 in cytoplasm and nuclear fractions were evaluated by western blot analysis;the mRNA expression of NF-κB p65 was analyzed by in situ hybridization (ISH). Results: Compared with the control group, the protein of NF-κB p65 both in cytoplasm and in nuclei was significantly higher than in I + MPP+ and MPP+ groups;similarly, the mRNA expression level of NF-κB p65 gene was also significantly higher;moreover, the protein expression of NF-κB p65 was much lower in I group (P + group, the protein of NF-κB p65 was significantly lower in I + MPP+ group, the mRNA expression level of NF-κB p65 gene was also significantly lower, and the protein expression level of NF-κB p65 was much lower in I + MPP+ group (P + group (P > 0.05). Conclusion: NF-κB activation is essential to MPP+-induced apoptosis in PC12 cells;but Isoflavone can inhibit the cell damage to some extent to execute its protective function, which may be involved in nigral neurodegeneration in patients with Parkinson’s disease.

Nuclear Factor kappa B p65 Expression in Mouse Cochlea

Nuclear factor kappa B(NF-κB) is one of the best-characterized transcription factors playing important roles in many cellular responses to a large variety of stimuli,including inflammatory cytokines, phorbol esters, growth factors, and bacterial and viral products. The aim of this study is to demonstrate NF-κB expression in the mouse cochlea and its enhancement in response to lipopolysaccharides(LPS) and kanamycin(KA) treatment. Methods KA treatment consisted of subcutaneous KA injections at 700 mg/kg twice a day with an eight-hour interval between the two injections for 3 or 7 days. For animals in the LPS treatment group, a single dose of 0.3 mg LPS dissolved in 0.2 ml sterile saline were injected into both bullae through the tympanic membrane and kept there for 3 hours. Animals in the control group received subcutaneous saline injection for 7 days. Following immmunohistochemichal processing with rabbit polyclonal anti-NF-κB p65 antibodies, cryosections of the cochlea were examined for expression of NF-κB p65 in various structures in the cochlea. Results NF-κB p65 expression, identified by presence of brown reaction products characteristic of DAB immunohistochemistry, was visible in the spiral ligament, spiral prominence, tectorial membrane(TM), spiral ganglion and nerve fibers. Relatively weak NF-κB p65 expression was also visualized in the organ of Corti. Within the organ of Corti, the inner hair cells(IHC), outer hair cells(OHC), inner pillar cells(IP), outer pillar cells (OP), Deiter’s cells(DC), and Boettcher’s cells exhibited stronger staining than the inner sulcus cells, Hensen’s cells(HC) and Claudius’cells. No NF-κB p65 expression was seen in the nucleus of the IHC and OHC. NF-κB p65 expression was increased in animals exposed to LPS or KA, demonstrating significant differences in the staining between control animals and LPS/KA-treated animals. NF-κB p65 expression was not significantly different between LPS treated and KA treated animals or between 3 and 7 days in KA-treated animals. Conclusion LPS and KA exposure increases expression of NF-κB p65 in the mouse cochlea.

人外周血单核细胞分化为树突状细胞过程中核转录因子-κBp50的表达及柴胡皂苷a的影响

目的观察人外周血单核细胞分化为树突状细胞(DC)过程中,核转录因子-κB p50(NF-κB p50)的表达以及柴胡皂苷a对单核细胞分化为树突状细胞的影响。方法非连续密度梯度离心获取人外周血单核细胞;用含粒单细胞刺激因子(GM-CSF)、IL-4、肿瘤坏死因子(TNF-α)和柴胡皂苷a的RPMI-1640培养液分别对细胞因子组、柴胡皂苷组、联合培养组的单核细胞进行体外培养;应用倒置相差显微镜、瑞氏染色和CD14、CD83、HLA-DR、S-100的免疫细胞化学法鉴定单核细胞和DC;动态观察单核细胞分化为DC过程中不同时间点的NF-κB p50的表达,并进行图像分析。结果CD14、CD83、HLA-DR、S-100免疫细胞化学法证实所获单核细胞和DC符合各自的形态和表型特征。在含GM-CSF和IL-4的RPMI-1640培养液培养7d时,单核细胞分化成未成熟DC(imDC);在含GM-CSF、IL-4和TNF-a的RPMI-1640培养液继续培养3d时,imDC分化为成熟DC(mDC),两者的细胞核内NF-κB p50表达具有显著性差异(P<0.05)。单纯用只含柴胡皂苷a的RPMI-1640培养液培养单核细胞至7d时,可见其细胞核呈NF-κBp50阳性,但未见其分化为DC。若用含GM-CSF、IL-4和柴胡皂苷a的RPMI-1640培养液联合培养7d时,则该单核细胞分化为imDC;加入TNF-α后继续培养3d,imDC的细胞核呈NF-κB p50强阳性,免疫细胞化学法证实imDC已经分化为mDC。联合培养组细胞的表型表达均强于只加细胞因子组(P<0.05)。结论人外周血单核细胞分化为imDC和mDC过程中,细胞核内NF-κB p50表达逐渐增强。单纯用低浓度柴胡皂苷a不能刺激单核细胞分化为DC,但联合细胞因子GM-CSF、IL-4和TNF-α培养时,可使其分化为imDC和mDC。

KLF5与NF-κB p50相互作用促进高糖诱导的血管平滑肌细胞炎症

目的探讨锌指转录因子Krüppel样因子5(Krüppel-like factor 5,KLF5)在高糖诱导的血管平滑肌细胞(vascular smooth muscle cells,VSMCs)炎症中的作用及机制。方法体外培养VSMCs,实时定量反转录聚合酶链反应(quantitative real-time polymerase chain reaction,qRT-PCR)、蛋白质印迹法(Western blot)检测高糖对VSMCs炎症基因肿瘤坏死因子α(tumor necrosis factor-α,TNF-α)、KLF5和核因子κB p50(nuclear factorκB p50,NF-κB p50)表达的影响。用小干扰RNA(small interfering RNA,siRNA)内源性敲低KLF5,Western blot检测VSMCs中TNF-α的表达。免疫共沉淀(co-immunoprecipitation,CoIP)检测VSMCs中高糖对KLF5和NF-κB p50相互作用的影响。结果qRT-PCR和Western blot结果显示,在mRNA和蛋白质水平,高糖显著上调炎症基因TNF-α、KLF5和NF-κB p50的表达,呈剂量及时间依赖性(P<0.05)。用siRNA内源性敲低KLF5后,高糖不能上调炎症基因TNF-α的表达。CoIP结果显示,高糖显著增强KLF5和NF-κB p50的相互作用。结论 KLF5通过与NF-κB p50相互作用促进高糖诱导的VSMCs炎症。

鼻息肉中核因子κB亚单位P50活性与IL-4、γ-IFN因子表达的关系

目的测定鼻息肉中核因子κB亚单位P50的活性及其与IL-4、γ-IFN表达的关系,探讨P50对TH1/TH2细胞因子表达调节的可能机制。方法采用SP免疫组化染色法检测40例鼻息肉患者与20例正常钩突黏膜中IL-4、γ-IFN、P50的表达,以核染阳性率来评估P50活性。对P50活性与IL-4,γ-IFN因子行直线相关分析。结果①鼻息肉中P50胞浆、胞核均有阳性表达,主要位于上皮细胞、炎症细胞及腺上皮细胞胞浆,P50活性显著增强(P<0.001),IL-4表达亦明显增强(P<0.001),γ-IFN表达无明显改变(P>0.05);②Pearson相关性分析提示,P50活性与IL-4表达呈直线正相关关系(r=0.70,P<0.001),而与γ-IFN表达无相关性(r=0.14,P=0.40)。结论鼻息肉中P50的活性明显增强,P50的激活上调IL-4的表达可能是鼻息肉中Th1/Th2因子失衡的重要环节之一。

甲状腺癌组织中NF-κBp65、NF-κBp50及HMGB1表达及意义

目的探讨甲状腺癌组织中核因子-κB(NF-κB)p65、NF-κB p50及高迁移率族蛋白B1(HMGB1)的表达水平及临床意义。方法选择解放军171医院2013年1月—2015年12月切取的甲状腺组织标本212例进行研究,其中甲状腺癌组织122例,甲状腺腺瘤组织30例,甲状腺肿组织30例,正常甲状腺组织30例,比较各组NF-κB p65、NF-κB p50及HMGB1表达,并分析其与甲状腺癌临床特征的关系,以及三者之间的相关性。结果甲状腺癌组、甲状腺腺瘤组和甲状腺肿组的HMGB1、NF-κB p50和NF-κB p65阳性率均高于正常甲状腺组(P<0.01),甲状腺癌组和甲状腺腺瘤组均高于甲状腺肿组(P<0.01),甲状腺癌组高于甲状腺腺瘤组(P<0.01)。肿瘤直径≥1.0 cm和有淋巴结转移的甲状腺癌组织中NF-κB p65、NF-κB p50及HMGB1表达阳性率高(P<0.01,P<0.05)。NF-κB p65、NF-κB p50及HMGB1三者间呈显著正相关(r=0.356、0.645和0.275,P<0.05)。结论甲状腺癌组织中NF-κB p65、NF-κB p50及HMGB1均呈高表达,并且与肿瘤直径和淋巴结转移有关。

葫芦巴碱调节PI3K/Akt/NF-κB信号通路对变应性接触性皮炎大鼠免疫反应的影响

目的探讨葫芦巴碱对变应性接触性皮炎(ACD)大鼠免疫、炎性反应及PI3K/Akt/NF-κB信号通路的影响。方法60只SD大鼠随机分为正常组、ACD组、葫芦巴碱(低、中、高)剂量组(20、40、80 mg/kg)和PI3K抑制剂(LY294002)组(40 mg/kg),每组10只。除正常组外,其余组大鼠采用2,4二硝基氟苯(DNFB)诱导ACD模型。给药结束后,通过录像观察大鼠挠痒行为;HE染色检测大鼠耳皮肤组织病理学变化;ELISA检测大鼠血清IgE及Th1、Th2、Th17型细胞因子(IFN-γ、IL-4、IL-17)水平;Western blot检测大鼠耳皮肤组织中炎性因子(IL-1β、IL-6)蛋白及PI3K/Akt/NF-κB信号通路相关蛋白表达。结果与正常组比较,ACD组大鼠挠痒次数增加,血清IgE、IFN-γ、IL-4、IL-17水平及耳皮肤组织中IL-1β、IL-6蛋白表达和p-PI3K/PI3K、p-Akt/Akt、p-NF-κB/NF-κB比值升高(P<0.05),耳皮肤组织角化过度且可见大量炎性细胞浸润;与ACD组比较,葫芦巴碱(低、中、高)剂量组和LY294002组大鼠挠痒次数减少,血清IgE、IFN-γ、IL-4、IL-17水平及耳皮肤组织中IL-1β、IL-6蛋白表达和p-PI3K/PI3K、p-Akt/Akt、p-NF-κB/NF-κB比值降低(P<0.05),耳皮肤组织病理损伤均有所改善,且葫芦巴碱各给药组呈剂量依赖效应;葫芦巴碱高剂量组和LY294002组大鼠上述指标比较,差异无统计学意义(P>0.05)。结论葫芦巴碱可抑制ACD大鼠皮肤组织中PI3K/Akt/NF-κB信号通路激活,调控Th1、Th2、Th17型免疫应答并减轻皮肤局部和全身炎性反应。

肝细胞癌中M2巨噬细胞标志物与NF-κB p50相关性研究

目的:探讨不同分期肝细胞癌病人组织中M2巨噬细胞及核因子κB (NF-κB)p50的表达情况,并分析其表达的相关性。方法:整群收集2012-2015年80例肝细胞肝癌病人和10例肝内胆管结石病人(对照组)的组织标本,采用免疫荧光双染法检测CD163和CD206的表达;收集2015年10月至2016年1月20例接受肝细胞癌手术病人的新鲜组织标本,采用Western blotting法检测不同分期的肝癌组织中CD163、CD206的表达及NF-κB p50的表达。结果:肝癌病人石蜡组织切片中CD163和CD206的共定位高于对照组,Ⅲ+Ⅳ期肝癌切片中的共定位高于Ⅰ+Ⅱ期;Western blotting结果表明,肝癌组织中CD163、CD206及NF-κB p50的表达高于癌旁组织(P<0.05～P<0.01),Ⅲ+Ⅳ期肝癌组织中的表达高于Ⅰ+Ⅱ期(P<0.01)。NF-κB p50与CD163、CD206的表达均呈正相关(r=0.963、0.944,P<0.01)。结论:随着肝癌进展,M2巨噬细胞数量和NF-κB p50的表达均升高,提示两者可能具有协同作用,共同促进肝癌进展。

Blocking NF-kB nuclear translocation leads to p53-related autophagy activation and cell apoptosis

AIM: To investigate the anti-tumor effects of nuclear factor-κB (NF-κB) inhibitor SN50 and related mechanisms of SGC7901 human gastric carcinoma cells. METHODS: MTT assay was used to determine the cytotoxic effects of SN50 in gastric cancer cell line SGC7901. Hoechst 33258 staining was used to detect apoptosis morphological changes after SN50 treatment. Activation of autophagy was monitored with monodansylcadaverine (MDC) staining after SN50 treatment.Immunofluorescence staining was used to detect the expression of light chain 3 (LC3). Mitochondrial membrane potential was measured using the fluorescent probe JC-1. Western blotting analysis were used to determine the expression of proteins involved in apoptosis and autophagy including p53, p53 upregulated modulator of apoptosis (PUMA), damage-regulated autophagy modulator (DRAM), LC3 and Beclin 1. We detected the effects of p53-mediated autophagy activation on the apoptosis of SGC7901 cells with the p53 inhibitor pifithrin-α. RESULTS: The viability of SGC7901 cells was inhibited after SN50 treatment. Inductions in the expression of apoptotic protein p53 and PUMA as well as autophagic protein DRAM, LC3 and Beclin 1 were detected with Western blotting analysis. SN50-treated cells exhibited punctuate microtubule-associated protein 1 LC3 in immunoreactivity and MDC-labeled vesicles increased after treatment of SN50 by MDC staining. Collapse of mitochondrial membrane potential Δψ were detected for 6 to 24 h after SN50 treatment. SN50-induced increases in PUMA, DRAM, LC3 and Beclin 1 and cell death were blocked by the p53 specific inhibitor pifithrin-α. CONCLUSION: The anti-tumor activity of NF-κB inhibitors is associated with p53-mediated activation of autophagy.

FAT10、NF-κB p50在乳腺浸润性导管癌中的表达及其临床意义

目的探讨双泛素(FAT10)和核因子-κB p50(NF-κB p50)在乳腺浸润性导管癌中的表达及其与临床病理特征的关系。方法应用Max VisionTM免疫组织化学法,检测112例乳腺浸润性导管癌组织和53例癌旁组织中FAT10与NF-κB p50的表达,并分析两者表达的相关性及其与乳腺癌临床病理特征的关系。结果 FAT10和NF-κB p50在乳腺浸润性导管癌中的阳性表达率分别为77.68%(87/112)和81.25%(91/112),明显高于癌旁组织的39.62%(21/53)和45.28%(24/53),差异均有统计学意义(P<0.001)。FAT10、NF-κB p50在乳腺浸润性导管癌中的表达与淋巴结转移、远处转移及TNM分期有关(P<0.05),而与患者的年龄、肿瘤大小及分子分型无关(P>0.05)。FAT10与NF-κB p50在乳腺浸润性导管癌中的表达呈显著正相关(r=0.624,P<0.001)。结论 FAT10、NF-κB p50的表达与乳腺浸润性导管癌的恶性程度及侵袭转移密切相关,两者可能共同促进肿瘤的发生发展。

PI3K/Akt/NF-κB通路调控ABCB1/P-gp介导的人结肠癌细胞多药耐药的研究

背景与目的:肿瘤的多药耐药(multidrug resistance,MDR)基因的表达是目前化疗失败的主要原因,磷脂酰肌醇-3-激酶(phosphoinositide 3-kinases,PI3K)信号通路参与肿瘤多药耐药的发生,但PI3K信号通路与多药耐药的机制尚不明确。本研究旨在探讨PI3K/Akt信号通路及其下游靶点对ATP结合蛋白亚家族1抗体(ATP-binding cassette sub-family B member 1,ABCB1)基因编码的P-糖蛋白(P-glycoprotein,P-gp)介导的人结肠癌耐奥沙利铂细胞株HCT-116/L-OHP细胞多药耐药性的调控作用。方法:将PI3K特异性抑制剂LY294002(20μmol/L)处理人结肠癌HCT-116/L-OHP细胞2 h后,用细胞计数试剂盒-8(cell counting kit-8,CCK-8)检测细胞对奥沙利铂的敏感性;蛋白质印迹法(Western blot)检测相关耐药蛋白P-gp、肺耐药蛋白(lung resistance-related protein,LRP)、多药耐药相关蛋白-2(multidrug resistance-related-2,MRP-2)以及PI3K/Akt信号通路下游蛋白Akt、p-Akt、IκB、p-IκB的表达变化;CHIP—PCR法检测核转录因子κB(NF-κB)对ABCB1基因启动子的影响。结果:阻断PI3K/Akt信号通路激活后,奥沙利铂对HCT-116/L-OHP细胞的半数抑制浓度(IC50)由(157.48±16.73)μg/mL降至(53.68±3.18)μg/mL,逆转指数为2.93(P<0.01)。HCT-116/L-OHP细胞的p-Akt、p-IκB和P-gp的表达水平明显下降(P<0.01),Akt、IκB、LRP和MRP-2表达变化不明显。NF-κB能够与ABCB1基因启动子区域结合。结论:阻断PI3K/AKT信号通路可增强人结肠癌HCT-116/L-OHP耐药细胞的药物敏感性,抑制p-Akt和p-IκB的磷酸化表达水平,逆转P-gp介导的肠癌多药耐药。

Modic Ⅱ型改变软骨终板中核因子-κB、白介素18和P物质的表达及意义

目的 ：观察核因子-κB（NF-κB）、白介素-18（IL-18）和P物质（SP）在ModicⅡ型改变软骨终板中的表达情况,并分析其意义。方法：收集2010年10月-2011年10月因单节段腰间盘退变性疾病行椎体间融合术的患者41例,男18例,女23例,年龄20-70岁,平均47.1±13.7岁。根据手术节段终板有无ModicⅡ型改变,将其分为ModicⅡ型改变组（A组）和无Modic改变组（B组）。同时收集因腰椎爆裂性骨折行前路手术治疗的5例年轻患者作为对照组（C组）,男3例,女2例,年龄20-29岁,平均24.2±3.7岁。对术中取出的软骨终板标本行HE染色观察软骨终板组织形态学变化,免疫组化法检测NF-κB、IL-18和SP表达阳性率及阳性细胞指数。结果：HE染色结果显示,C组软骨终板无明显退变,A组退变程度重于B组。免疫组化结果显示,A、B、C组NF-κB阳性细胞指数分别为55.39±17.74、36.01±14.80、4.42±2.84,IL-18阳性细胞指数分别为45.23±12.95、30.22±12.01、5.22±3.46,SP阳性细胞指数分别为38.29±19.26、25.83±16.52、0.97±1.32。A、B组NF-κB、IL-18和SP阳性细胞指数均明显高于C组（P〈0.05）,A组明显高于B组（P〈0.05）,NF-κB与IL-18的表达水平呈高度正相关关系（P〈0.05）。结论：ModicⅡ型改变软骨终板中NF-κB、IL-18和SP表达的阳性细胞数显著性升高,可能是ModicⅡ型改变引起腰痛的原因之一。

核因子-κB对癫痫大鼠脑P-糖蛋白表达的调控作用

目的探讨核因子-κB(NF-κB)对癫痫大鼠脑P-糖蛋白(P-gp)表达的影响。方法将雄性SD大鼠随机分为假手术组(n=9)、癫痫组(EP组,n=14)、NF-κB活性抑制剂吡咯烷二硫代氨基甲酸盐(PDTC)干预组(PDTC组,n=14)。采用大鼠海马注射海人酸方法制作癫痫模型,PDTC组于癫痫造模前30 min给予腹腔注射PDTC(按体质量150 mg/kg)。于造模后24 h处死各组大鼠,采用免疫组织化学方法检测并比较各组大鼠海马CA3区、齿状回、嗅周皮层、杏仁核复合体区P-gp和NF-κB亚基p65(NF-κBp65)表达情况。结果与假手术组相比,EP组海马CA3区、齿状回、杏仁核复合体区P-gp和NF-κBp65表达显著增强(P<0.01),PDTC组P-gp和NF-κBp65表达低于EP组(P<0.01),且二者具有正等级相关性(P<0.05),而在嗅周皮层二者无相关性(P>0.05)。结论抑制NF-κB活化可以降低癫痫相关脑区P-gp过表达,癫痫发作所致脑内P-gp表达上调可能与NF-κB活化有关。

雷公藤红素下调p-p38、p-JNK、NF-κB减轻脑梗死后的炎症反应

目的探讨脑缺血后磷酸化p38丝裂原活化蛋白激酶(p-p38)、磷酸化c-Jun氨基末端激酶(p-JNK)、核因子-κB(NF-κB)的表达变化,观察雷公藤红素的脑保护作用及机制。方法用改良线栓法制备大鼠大脑中动脉永久性脑梗死(pMCAO)模型。实验分为3组:溶剂对照组,假手术组和雷公藤红素组(3mg·kg^(-1)腹腔注射)。采用RT-qPCR和Western blot观察p-p38、p-JNK、NF-κB基因和蛋白表达变化,比较各组的患侧脑水肿、脑梗死体积和神经功能评分。结果与溶剂对照组相比,雷公藤红素组脑水肿明显低于溶剂对照组(P<0.05);梗死体积明显小于溶剂对照组(P<0.05);神经功能评分明显小于溶剂对照组(P<0.05);p-p38、p-JNK、NF-κB的表达明显低于溶剂对照组(P<0.05)。结论雷公藤红素对脑梗死大鼠具有脑保护作用,雷公藤红素通过调节p-p38,p-JNK和NF-κB的表达可能是其脑保护作用机制之一。

阿维A对P物质诱导的HaCaT细胞NF-κB表达的影响

目的:明确阿维A对HaCaT细胞NF-κB表达的影响。方法:细胞共分5组:对照组、单纯P物质刺激组、P物质+小剂量阿维A组、P物质+中剂量阿维A组、P物质+大剂量阿维A组。应用免疫细胞化学法、Western-blot和RT-PCR法检测各组HaCaT细胞中NF-κB阳性细胞表达率、细胞蛋白和基因表达的变化。结果:单纯P物质刺激组较对照组阳性细胞表达率、细胞蛋白、mRNA表达均增强。各阿维A剂量组较P物质组阳性细胞表达率、蛋白和mRNA表达均降低(P<0.05或P<0.01)。结论:阿维A对人角质形成细胞NF-κB的调控是其治疗皮肤病的作用途径之一。

NF-κB抑制剂PDTC逆转K562/AO_2细胞耐药性及其机制的研究

为研究NF-κB的异常活化在K562/AO2细胞耐药机制中的作用,采用非细胞毒剂量抗氧化剂吡咯烷二硫代氨基甲酸盐(PDTC)抑制K562/AO2细胞NF-κB表达,用MTT法检测K562/AO2细胞对药物敏感性的变化,RT-PCR、流式细胞术分别检测K562、K562/AO2细胞mdr-1 mRNA、P-gp表达水平以及不同浓度PDTC作用一定时间对其影响。结果显示:①阿霉素(ADM)诱导耐药的K562/AO2细胞对ADM的耐药性是K562细胞的59倍;非细胞毒剂量PDTC预作用后,ADM对K562/AO2细胞的IC50显著降低,相对逆转耐药效率为93.03%,强于经典耐药逆转剂维拉帕米(Ver);②K562/AO2细胞NF-κB表达水平高于K562细胞(p<0.01);3组非细胞毒剂量PDTC作用后K562/AO2细胞NF-κB表达均受抑制;0.2μmol/LPDTC作用24小时抑制效应最强,K562/AO2细胞NF-κB表达降至接近K562细胞水平(p>0.05);③K562/AO2细胞mdr-1 mRNA、P-gp表达均高于K562细胞(p<0.01);3组非细胞毒剂量PDTC作用K562/AO2细胞48小时后,其mdr-1 mRNA、P-gp表达明显减少。结论:抑制NF-κB异常活化可部分逆转K562/AO2细胞耐药性,其机制与mdr-1 mRNA及其编码的P-gp表达减少有关。

PCV2感染对仔猪肝脏MyD88-NF-κB信号途径的影响

选取31头经检测猪圆环病毒2型(PCV2)、猪繁殖与呼吸综合征病毒(PRRSV)抗原和抗体均为阴性的5周龄断奶仔猪,随机分为对照组16头和试验组15头,对照组仔猪每头滴鼻4 mL PBS,试验组仔猪每头滴鼻4 mL 5×105TCID50.mL-1PCV2悬液。于PCV2接种当天剖杀4头仔猪作为对照组,分别于14、21和35 d剖杀4头对照组和5头试验组仔猪,采集肝脏。用激光共聚焦显微镜检测核因子κB/P65(NF-κB/P65)蛋白的核易位变化;蛋白提取法分别提取肝脏细胞核蛋白和胞浆蛋白,Western blot定量检测细胞核中NF-κB/P65和细胞浆中p-IκBα、MyD88蛋白含量的变化;电泳迁移率(EMSA)法检测细胞核中NF-κB DNA的结合率变化。检测结果显示,PCV2接种仔猪,肝脏中NF-κB/P65蛋白核易位逐渐增多,到21 d达到峰值;p-IκBα、MyD88、NF-κB/P65 DNA结合率在接种后均先升高后趋于恢复,并于21 d达到高峰。与对照组仔猪相比,肝脏中MyD88和NF-κB/P65蛋白含量以及NF-κB DNA结合率在14和21 d试验组均显著升高(P<0.05),35 d含量变化不显著;21 d时试验组p-IκBα蛋白含量显著升高。相关性分析显示,NF-κB/P65蛋白含量与MyD88含量、NF-κB DNA结合率之间存在显著正相关,相关系数分别是0.566和0.528。结果表明,PCV2可通过激活MyD88启动NF-κB信号途径;通过IκBα的磷酸化降解激活NF-κB,并促进其进行核易位,使NF-κB与DNA发生结合,调控相关炎性细胞因子的转录和表达。