Macrophage inflammatory protein-2 as mediator of inflammation in acute liver injury

Macrophage inflammatory protein(MIP)-2 is one of the CXC chemokines and is also known as chemokine CXC ligand(CXCL2). MIP-2 affects neutrophil recruitment and activation through the p38 mitogen-activatedprotein-kinase-dependent signaling pathway, by binding to its specific receptors, CXCR1 and CXCR2. MIP-2 is produced by a variety of cell types, such as macrophages, monocytes, epithelial cells, and hepatocytes, in response to infection or injury. In liver injury, activated Kupffer cells are known as the major source of MIP-2. MIP-2-recruited and activated neutrophils can accelerate liver inflammation by releasing various inflammatory mediators. Here, we give a brief introduction to the basic molecular and cellular sources of MIP-2, and focus on its physiological and pathological functions in acute liver injury induced by concanavalin A, lipopolysaccharides, irradiation, ischemia/reperfusion, alcohol, and hypoxia, and hepatectomy-induced liver regeneration and tumor colorectal metastasis. Further understanding of the regulatory mechanisms of MIP-2 secretion and activation may be helpful to develop MIP-2-targeted therapeutic strategies to prevent liver inflammation.

Th17/Treg balance and macrophage polarization ratio in lower extremity arteriosclerosis obliterans

Objective:To explore the balance of peripheral blood T helper 17 cells/regulatory T cell(Th17/Treg)ratio and the polarization ratio of M1 and M2 macrophages in lower extremity arteriosclerosis obliterans(ASO).Methods:A rat model of lower extremity ASO was established,and blood samples from patients with lower extremity ASO before and after surgery were obtained.ELISA was used to detect interleukin 6(IL-6),IL-10,and IL-17.Real-time RCR and Western blot analyses were used to detect Foxp3,IL-6,IL-10,and IL-17 expression.Moreover,flow cytometry was applied to detect the Th17/Treg ratio and M1/M2 ratio.Results:Compared with the control group,the iliac artery wall of ASO rats showed significant hyperplasia,and the concentrations of cholesterol and triglyceride were significantly increased(P<0.01),indicating the successful establishment of ASO.Moreover,the levels of IL-6 and IL-17 in ASO rats were pronouncedly increased(P<0.05),while the IL-10 level was significantly decreased(P<0.05).In addition to increased IL-6 and IL-17 levels,the mRNA and protein levels of Foxp3 and IL-10 in ASO rats were significantly decreased compared with the control group.The Th17/Treg and M1/M2 ratios in the ASO group were markedly increased(P<0.05).These alternations were also observed in ASO patients.After endovascular surgery(such as percutaneous transluminal angioplasty and arterial stenting),all these changes were significantly improved(P<0.05).Conclusions:The Th17/Treg and M1/M2 ratios were significantly increased in ASO,and surgery can effectively improve the balance of Th17/Treg,and reduce the ratio of M1/M2,and the expression of inflammatory factors.

Toxoplasma ROP16Ⅰ/Ⅲ ameliorated inflammatory bowel diseases via inducing M2 phenotype of macrophages

BACKGROUND Inflammatory bowel disease(IBD)is characterized by chronic and non-specific inflammation of the intestinal mucosa and mainly includes ulcerative colitis and Crohn's disease.AIM To explore the beneficial effect of ToxoROP16I/III-induced M2 phynotype macrophages in homeostasis of IBDs through downregulation of M1 inflammatory cells.METHODS RAW264.7 macrophages stimulated by lipopolysaccharide(LPS)(M1 cells)were co-cultured with Caco-2 cells as an inflammatory model of IBD in vitro.The expression of ToxoROP16I/III was observed in RAW264.7 macrophages that were transfected with pEGFP-rop16I/III.The phenotypes of M2 and M1 macrophage cells were assessed by quantitative real-time reverse transcriptase polymerase chain reaction and the expression of tumor necrosis factor(TNF)-α,interleukin(IL)-1β,IL-6,transforming growth factor(TGF)-β1,IL-10,inducible nitric oxide synthase(iNOS),and arginase-1(Arg-1)was detected.The expression of iNOS,Arg-1,signal transducer and activator of transcription 3(Stat3),p-Stat3,Stat6,p-Stat6,programmed death ligand-2(PD-L2),caspase-3,-8,and-9 was analyzed by Western blotting,and Griess assays were performed to detect nitric oxide(NO).TNF-α,IL-1β,IL-6,TGF-β1,and IL-10 expression in the supernatants was detected by enzyme-linked immunosorbent assay,and Caco-2 cell apoptosis was co-culture system.RESULTS M1 cells exhibited significantly increased production of iNOS,NO,TNF-α,IL-1β,and IL-6,while ToxoROP16I/III induced macrophage bias to M2 cells in vitro,showing increased expression of Arg-1,IL-10 and TGF-β1 and elevated production of p-Stat3 and p-Stat6.The mixed M1 and M2 cell culture induced by ToxoROP16I/III exhibited decreased production of NO and iNOS and upregulated expression of Arg-1 and PD-L2.Accordingly,Caco-2 cells became apoptotic,and apoptosis-associated proteins such as caspase-3,-8 and-9 were dampened during co-culture of M1 and M2 cells.Flow cytometry analysis showed that co-culture of M1 cells with Caco-2 cells facilitated the apoptosis of Caco-2 cells,but co-culture of M1 and M2 cells alleviated Caco-2 cell apoptosis.CONCLUSION ToxoROP16I/III-induced M2 macrophages inhibited apoptosis of Caco-2 cells caused by M1 macrophages.This finding may help gain a better understanding of the underlying mechanism and represent a promising therapeutic strategy for IBDs.

The Expression of Interleukin-17, Interferon-gamma, and Macrophage Inflammatory Protein-3 Alpha mRNA in Patients with Psoriasis Vulgaris

Summary: To investigate the role of Interleukin-17 (IL-17), Interferon-gamma (IFN-γ), and macrophage inflammatory protein-3 alpha (MIP-3α) in the pathogenesis of psoriasis, reverse transcriptase-polymerase chain reaction (RT-PCR) was used to semi-quantitatively analyze the mRNA expression of IL-17, IFN-γ, and MIP-3α in 31 psoriatic lesions and 16 normal skin tissues. The results showed that the mRNA of the three cytokines was present in all specimens. And the expression level of IL-17 mRNA in skin lesions was 1.1416±0.0591, which was significantly higher than that in normal controls (0.8788±0.0344, P<0.001). The expression levels of IFN-γ mRNA were 1.1142±0.0561 and 0.9050±0.0263, respectively, with significant difference(P<0.001). And the expression levels of MIP-3α mRNA in psoriatic lesions was 1.1397±0.0521, which was markedly higher than that in normal controls (0.8681±0.0308, P<0.001). These findings indicate that up-regulated expression of IL-17, IFN-γ, and MIP-3α might be involved in the pathogenesis of psoriasis.

Macrophage Inflammatory Protein-1 Beta (MIP-1<i>β</i>) and Platelet Indices as Predictors of Spontaneous Bacterial Peritonitis<br>—MIP, MPV and PDW in SBP

Background/Aims: The objective of this study is to measure macrophage inflammatory protein one beta (MIP-1β), mean platelet volume (MPV) and platelet distribution width (PDW) to evaluate their usefulness in the diagnosis of spontaneous bacterial peritonitis (SBP) in cirrhotic patients. Materials and Methods: This study comprised 41 cirrhotic patients with ascites. MPV, PDW and MIP-1β were measured in serum and ascitic fluid. Results: A significant increase MPV, PDW, C-reactive Protein (CRP) and white blood cell was observed in SBP group compared to non SBP (P ≤ 0.001, P = 0 β was significantly in-creased in ascitic fluid in patients with SBP versus non SBP (P ≤ 0.001). At cutoff value of 8.3 fl MPV had 85.7% sensitivity and 75% specificity (AUC = 0.876) for diagnosis of SBP. At cutoff value of 15.4 PDW had 90.4% sensitivity and 55% specificity (AUC = 0.762). At cutoff value of 121.9 pg/ml MIP-1β in ascitic fluid had 76.1% sensitivity and 100% specificity (AUC = 0.881) for detecting SBP. Conclusion: MIP-1β and platelet indices are useful marker in the diagnosis of SBP in cirrhotic patients. Combined measurement of MIP-1β in serum and ascitic fluid had 100% sensitivity and specificity for diagnosis of SBP.

miRNA调控claudin-2表达对溃疡性结肠炎小鼠巨噬细胞极化的机制

目的探讨微小核糖核酸(MicroRNA,miRNA)通过封闭蛋白2(Recombinant,claudin-2)表达变化对溃疡性结肠炎小鼠的保护作用及对巨噬细胞极化的调控。方法选取BALB/c雌性小鼠按照体重随机分成对照组、模型组以及上调组和下调组,每组15只。对4组小鼠溃疡性结肠组织进行HE染色,观察分析小鼠溃疡性结肠炎评分情况、炎性因子、免疫细胞、巨噬细胞、claudin-2表达。结果与对照组比较,模型组、上调组、下调组miRNA表达升高(P<0.05);与模型组比较,上调组miRNA表达降低、下调组升高(P<0.05);与上调组比较,下调组miRNA表达升高(P<0.05);与模型组比较,上调miRNA第3 d、5 d、7 d的溃疡性结肠炎模型小鼠明显降低、下调组升高;与上调组比较,下调组miRNA表达升高(P<0.05);与对照组比较,模型组、上调组、下调组T淋巴细胞的糖蛋白(CD4^(+))、白细胞分化抗原(CD8^(+))水平升高(P<0.05);与模型组比较,上调组CD4^(+)、CD8^(+)水平降低,下调组升高(P<0.05);与上调组比较,下调组CD4^(+)、CD8^(+)水平升高(P<0.05);与对照组比较,模型组、上调组、下调组肿瘤坏死因子(TNF-α)、白介素-6(IL-6)、白介素-8(IL-8)水平升高(P<0.05);与模型组比较,上调组TNF-α、IL-6、IL-8水平降低(P<0.05);与上调组比较,下调组升高(P<0.05);与对照组比较,模型组、上调组、下调组诱导型一氧化氮合酶(iNOS)水平升高,巨噬细胞甘露糖受体(CD206)降低(P<0.05);与模型组比较,上调组iNOS水平降低、CD206水平升高,下调组iNOS水平升高、CD206水平降低(P<0.05);与上调组比较,下调组iNOS升高、CD206降低(P<0.05);与对照组比较,模型组、上调组、下调组claudin-2蛋白表达升高(P<0.05);与模型组比较,上调组claudin-2蛋白表达降低、下调组claudin-2蛋白表达升高(P<0.05)。结论上调溃疡性结肠炎小鼠miRNA能够调节巨噬细胞极化,从而改善溃疡性结肠炎小鼠。

2型糖尿病患者血清巨噬细胞炎症蛋白1α和基质金属蛋白酶9水平与甲状腺结节的相关性研究

目的探讨2型糖尿病(T_(2)DM)患者血清巨噬细胞炎症蛋白1α(MIP-1α)、基质金属蛋白酶9(MMP-9)水平与甲状腺结节的相关性。方法回顾性选取2021年10月至2023年3月于河北医科大学第三医院就诊的T_(2)DM患者154例,根据患者是否合并甲状腺结节分为甲状腺结节组(83例)和无甲状腺结节组(71例)。比较2组甲状腺功能、血糖、血脂、MIP-1α、MMP-9等指标。采用Logistic回归模型分析影响T_(2)DM患者出现甲状腺结节的因素;采用Pearson相关性检验分析T_(2)DM患者血清MIP-1α、MMP-9水平与其他因素的相关性;绘制受试者工作特征曲线分析血清MIP-1α、MMP-9水平对T_(2)DM患者出现甲状腺结节的预测价值。结果甲状腺结节组促甲状腺激素(TSH)、总三碘甲状腺原氨酸(TT_(3))、总甲状腺素(TT_(4))、稳态模型胰岛素抵抗指数(HOMA-IR)、稳态模型胰岛β细胞功能指数、空腹血糖、空腹胰岛素水平均高于无甲状腺结节组,胰岛素敏感指数(ISI)低于无甲状腺结节组(均P<0.05)。甲状腺结节组血清MIP-1α、MMP-9水平均高于无甲状腺结节组[(29±5)ng/L比(25±5)ng/L、(2.0±0.5)ng/L比(1.4±0.5)ng/L](均P<0.001)。Logistic回归分析结果显示,MIP-1α、MMP-9、TSH、TT_(3)、TT_(4)、空腹胰岛素、HOMA-IR和ISI均为T_(2)DM患者出现甲状腺结节的危险因素(均P<0.05)。Pearson相关性分析结果表明,T_(2)DM患者血清MIP-1α与MMP-9水平呈正相关(r=0.362,P<0.001)。血清MIP-1α、MMP-9水平与空腹胰岛素、TSH、HOMA-IR、TT_(3)、TT_(4)均呈正相关,与ISI呈负相关(均P<0.001)。MIP-1α、MMP-9水平联合检测预测T_(2)DM患者出现甲状腺结节的曲线下面积大于MIP-1α、MMP-9单独检测(均P<0.05)。结论血清MIP-1α、MMP-9水平与T_(2)DM患者出现甲状腺结节具有密切关系,对预测T_(2)DM患者甲状腺结节具有重要价值。

巨噬细胞上髓系细胞触发受体-1/2在炎症性肠病中的作用研究进展

炎症性肠病(inflammatory bowel disease,IBD)是以克罗恩病(Crohn’s disease,CD)和溃疡性结肠炎(ulcerative colitis,UC)为代表的慢性肠道炎症性疾病,机制涉及遗传易感性以及环境与微生物群间相互作用削弱肠道屏障导致免疫激活等多种途径。近年来,巨噬细胞上表达的TREMs(triggering receptors expressed on myeloid cells),即髓系细胞触发受体,被发现在固有免疫和适应性免疫中发挥重要作用,并与IBD的发生发展密切相关。本文将着重对TREM-1/2(TREM-1和TREM-2)的结构、配体和作用,其在巨噬细胞上参与IBD与伴发精神障碍的机制研究进行概述,旨在为IBD的预防和治疗提供理论支持。

Expression of Macrophage Inflammatory Protein 1α in the Endothelial Cells Exposed to Diamide

In order to study whether the endothelial cells (ECs) with lipid peroxidation induced by diamide can express and secrete macrophage inflammatory protein 1α (MIP-1α), the expression of MIP-1α protein in the cells was detected by cell enzyme-linked immunosorbent assay (ELISA) and that of MIP-1α mRNA was determined by cell in situ hybridization and nuclease S1 protection assay after the ECs were exposed to different concentrations of diamide for 4 h. The chemotactic activity of MIP-1α was tested by micropore filter method using modified Boyden chambers. Cell ELISA showed that the expression of MIP-1α protein in endothelial cells exposed to 1 μmol/L, 5 μmol/L and 10 μmol/L diamide was 1.9-fold, 2.3-fold and 1.7-fold respectively as much as that in the control cells, which was statistically significant by analysis of variance. In situ hybridization revealed that the mRNA expression of ECs treated with 1 μmol/L, 5 μmol/L and 10 μmol/L diamide was 1 3-fold, 3.0-fold and 1.7-fold as much as that in the control group, which had statistical significance ( F =188.93, P <0.01). The mRNA expression in 5 μmol/L dimide treated ECs, measured by nuclease S1 protection assay, was 3.4-fold as much as that in the control group( t =8 70, P <0 05). Chemotactic response(99.50±4.31 μm) to the culture medium conditioned by 5 μmol/L diamide treated ECs , which was stronger than that(66.47±3.25 μm) conditioned by the ECs ( F =404.31, P <0.05), was significantly decreased ( F =192.25, P <0.05) after adding MIP-1α antibody. It suggests that diamide, a lipid peroxidation inducer, could stimulate ECs to produce high level of MIP-1α, and might play an important role in atherogenesis by promoting the migration of peripheral blood monocytes into arterial intima.

Role of monocytes and macrophages in experimental and human acute liver failure

Acute liver failure (ALF) is a devastating clinical syndrome characterised by progressive encephalopathy, coagulopathy, and circulatory dysfunction, which commonly leads to multiorgan failure and death. Central to the pathogenesis of ALF is activation of the immune system with mobilisation of cellular effectors and massive production of cytokines. As key components of the innate immune system, monocytes and macrophages are postulated to play a central role in the initiation, progression and resolution of ALF. ALF in humans follows a rapidly progressive clinical course that poses inherent difficulties in delineating the role of these pivotal immune cells. Therefore, a number of experimental models have been used to study the pathogenesis of ALF. Here we consider the evidence from experimental and human studies of ALF on the role of monocytes and macrophages in acute hepatic injury and the ensuing extrahepatic manifestations, including functional monocyte deactivation and multiple organ failure.

发育型内皮基因座-1作用下氧化型低密度脂蛋白对巨噬细胞分泌TNF-α、MIP-1α及MIP-2的影响

目的探讨发育型内皮基因座-1(DEL-1)作用下氧化型低密度脂蛋白(OX-LDL)对巨噬细胞中肿瘤坏死因子α(TNF-α)、巨噬细胞炎性蛋白1α(MIP-1α)及巨噬细胞炎性蛋白2(MIP-2)表达的影响。方法体外培养人单核-巨噬细胞系THP-1细胞株至对数生长期,分为佛波脂(PMA)组(PMA诱导为贴壁的巨噬细胞)、OX-LDL组(OX-LDL诱导为泡沫细胞)、si-NC组(50 nmol/L siRNA-NC的小干扰转染细胞)及小干扰RNA-DEL-1(siRNA-DEL-1)组(50 nmol/L siRNA-DEL-1转染细胞),采用油红O染色鉴定泡沫细模型、并检测各组细胞中脂质积累,采用免疫荧光技术检测各组细胞中DEL-1的表达,采用实时聚合酶链反应(RT-PCR)及Western blot检测各组细胞中DEL-1、MIP-1α、MIP-2及TNF-α信使RNA(mRNA)和蛋白的表达;采用Pearson相关系数分析DEL-1蛋白表达与上述炎性因子的相关性。结果油红O染色结果显示,靶向敲低DEL-1泡沫细胞胞质内脂质积累减少;免疫荧光、Western blot及RT-PCR结果显示,OX-LDL组、siRNA-NC组细胞中DEL-1及下游炎性因子MIP-1α、MIP-2及TNF-α的蛋白及mRNA表达较PMA组上调(P<0.05),siRNADEL-1组细胞中上述因子表达较OX-LDL组及siRNANC组下调(P<0.05)。结论DEL-1介导了OX-LDL源性泡沫细胞分泌MIP-1α、MIP-2及TNF-α,可能参与了动脉粥样硬化(AS)的病变过程。

刺槐素对小鼠骨髓巨噬细胞AIM2炎症小体活化的抑制作用

目的 探讨刺槐素对脂多糖(LPS)和双链DNA模拟物poly(dA:dT)共诱导的小鼠骨髓巨噬细胞(BMDMs)黑色素瘤缺乏因子2(AIM2)炎症小体活化的影响。方法 在小鼠股骨中分离并培养BMDMs,将其分为对照组、LPS组、LPS+poly(dA:dT)组和LPS+poly(dA:dT)+刺槐素组。对照组将BMDMs继续在完全培养基中培养3 h;LPS组将BMDMs在加入含50 ng/mL LPS的完全培养基中培养3 h;LPS组+poly(dA:dT)组将BMDMs在加入含50 ng/mL LPS的完全培养基中培养3 h,再加入poly(dA:dT) 10μmol/L作用0.5 h;LPS+poly(dA:dT)+刺槐素组将BMDMs在加入含50 ng/mL LPS的完全培养基中培养3 h,然后加入刺槐素10μmol/L作用0.5 h,最后加入poly(dA:dT) 10μmol/L作用0.5 h。采用Western blotting法检测细胞裂解液pro-Caspase-1、pro-白细胞介素(IL)-1β和上清液Caspase-1、IL-1β蛋白相对表达量,ELISA法检测细胞上清液IL-1β、IL-18、TNF-α蛋白表达,乳酸脱氢酶(LDH)法检测细胞上清液LDH浓度。结果 各组细胞裂解液pro-Caspase-1、pro-IL-1β蛋白相对表达量比较差异均无统计学意义(P均>0.05)。与对照组、LPS组比较,LPS+poly(dA:dT)组和LPS+poly(dA:dT)+刺槐素组上清液Caspase-1、IL-1β蛋白相对表达量均升高,且LPS+poly(dA:dT)组升高更明显(P均<0.05)。与对照组、LPS组比较,LPS+poly(dA:dT)组和LPS+poly(dA:dT)+刺槐素组细胞上清液IL-1β、IL-18蛋白表达均升高,且LPS+poly(dA:dT)组IL-1β升高更明显(P均<0.05)。与对照组比较,LPS组、LPS+poly(dA:dT)组和LPS+poly(dA:dT)+刺槐素组细胞上清液TNF-α蛋白表达及LDH水平均升高,且LPS+poly(dA:dT)组和LPS+poly(dA:dT)+刺槐素组升高更明显(P均<0.05)。结论 刺槐素对小鼠BMDMs的AIM2炎症小体活化具有抑制作用,能够减少细胞中Caspase-1、IL-1β蛋白表达,从而减轻炎症反应。

肠绞痛患儿血清sIL-2R、IFN-β、MIP-1β水平分析及与肠道菌群丰度的相关性

目的探讨肠绞痛患儿血清可溶性白细胞介素2受体(sIL-2R)、干扰素-β(IFN-β)、巨噬细胞炎性蛋白1β(MIP-1β)水平及与肠道菌群丰度的相关性。方法选择2020年1月—2022年1月本院收治的肠绞痛患儿120例作为观察组;另选择同期健康婴儿100名作为对照组。比较两组肠道菌群丰度、代谢指标、血清sIL-2R、IFN-β、MIP-1β水平差异。结果观察组双歧杆菌、韦荣球菌、萨特菌属、链球菌属和乳酸菌属丰度分别为0.79(0.68,0.92)、2.30(1.70,2.98)、0.77(0.62,0.90)、24.49(23.10,29.30)和11.10(9.30,12.80),明显高于对照组(P<0.05),而埃格特菌属、肠球菌属丰度分别为0.08(0.06,0.12)和5.10(4.30,6.70),明显低于对照组(P<0.05)。观察组乙酸为(3.19±0.92)mmol/L,明显低于对照组(P<0.05),丙酸、丁酸、异丁酸、戊酸、异戊酸分别为(1.20±0.21)mmol/L、(1.16±0.34)mmol/L、(1.23±0.19)mmol/L、(1.11±0.24)mmol/L和(1.09±0.21)mmol/L,明显高于对照(P<0.05)。观察组血清sIL-2R和MIP-1分别为(44.40±12.43)pg/ml和(110.40±31.12)pg/ml,明显高于对照组(P<0.05),而IFN-β为(33.10±11.43)pg/ml,明显低于对照组(P<0.05)。血清sIL-2R、MIP-1β与双歧杆菌属丰度呈正相关(P<0.05),而与肠球菌属丰度呈负相关(P<0.05)。血清IFN-β与双歧杆菌属丰度呈负相关(P<0.05),而与肠球菌属丰度呈正相关(P<0.05)。观察组治疗后双歧杆菌、韦荣球菌、萨特菌属、链球菌属、乳酸菌属丰度、丙酸、丁酸、异丁酸、戊酸、异戊酸、sIL-2R和MIP-1β明显低于治疗前(P<0.05),而埃格特菌属、肠球菌属丰度、乙酸、IFN-β明显高于治疗前(P<0.05)。结论肠绞痛患儿血清sIL-2R和MIP-1β水平升高,IFN-β水平降低,三者水平与双歧杆菌属、肠球菌属丰度呈相关性,值得进一步研究。

机械牵张诱导肺泡巨噬细胞的细胞因子表达谱及其与脂多糖对MIP-2释放的协同效应

目的观察机械牵张诱导肺泡巨噬细胞（AM）的细胞因子表达谱，以及机械牵张对脂多糖（LPS）诱导巨噬细胞炎性蛋白2（MIP-2）表达的影响。方法用LiquiChip液相蛋白芯片系统检测机械牵张诱导AM15种细胞因子的水平变化；检测不同强度机械牵张（5％、10％、15％和20％）和牵张刺激（20％）后不同时间点（0、1、3、6、12和24h）AM分泌MIP-2的水平，以及机械牵张（20％）与LPS（10ng／mL）共同刺激对AM分泌MIP-2的影响。结果牵张刺激后AM分泌IL-1β、IL-6、MIP-2、单核细胞趋化蛋白1（MCP-1）、IFN-γ和干扰素诱导蛋白10（IP-10）的水平明显升高（P均〈0．001）。机械牵张以强度和时间依赖方式诱导MIP-2的分泌，随着牵张强度的增加（10％、15％和20％），MIP-2的分泌水平也明显增加（P均〈0．001）；在刺激后6～24h范围内MIP-2水平持续升高（P〈0．001）。以机械牵张和LPS共同刺激AM，MIP-2的生成量大大增加，二者存在协同效应（F=121．983，P〈0．001）。结论机械牵张可诱导AM释放多种细胞因子，机械牵张诱导MIP-2的上调具有强度和时间依赖性，并协同LPS诱导AM释放MIP-2，可能在呼吸机所致肺损伤的发生和发展中起重要作用。

血清巨噬细胞炎症蛋白-2在脓毒症患者病情严重程度及预后中的评估价值

目的探讨脓毒症患者早期血清巨噬细胞炎症蛋白-2(macrophage inflammatory protein-2,MIP-2)的浓度、急性生理学与慢性健康状况评分系统Ⅱ(APACHEⅡ)评分、降钙素原(procalcitonin,PCT)动态变化及与预后的关系。方法采用前瞻性研究方法,选择2011年3月至2012年9月重症监护病房(ICU)62例脓毒症患者,按照目标导向治疗(EGDT)方案进行复苏,将完成6 h EGDT复苏目标者归为Ⅰ组,未完成6 h EGDT复苏目标者归为Ⅱ组。分别记录患者复苏前(T0),复苏后6 h(T6 h)及复苏后1 d(T1 d)、2 d(T2 d)、3 d(T3 d)、4 d(T4 d)、5 d(T5 d)的APACHEⅡ评分,检测患者血中MIP-2、PCT、尿素氮(BUN)及肌酐(Cr)等指标动态变化。根据患者28 d转归分为存活组和死亡组。结果Ⅰ组APACHEⅡ评分、血MIP-2、PCT及BUN、Cr于复苏成功后呈逐渐下降趋势,于T5 d最低;Ⅱ组APACHEⅡ评分、血MIP-2、PCT及BUN、Cr于复苏失败后呈逐渐上升趋势;Ⅱ组APACHEⅡ评分于T2 d时,血MIP-2于T1 d时较Ⅰ组明显升高(均P<0.05)。Ⅰ组死亡率明显低于Ⅱ组[12.5%(5/40)vs 68.2%(15/22),P<0.05]。存活组APCHEⅡ评分、血MIP-2、PCT及血BUN、Cr随病情好转逐渐下降,于T5 d最低,而死亡组则显著上升;死亡组APACHEⅡ评分于T1 d时、血MIP-2于T6 h时即较存活组明显升高(均P<0.05)。结论 MIP-2是评估脓毒症的良好指标,动态监测其变化可了解脓毒症的发展过程,结合APACHEⅡ评分及PCT变化,对疾病的严重程度及预后有重要的评估意义。

吸烟诱导的慢性支气管炎大鼠模型巨噬细胞炎性蛋白-2及髓过氧化物酶研究

目的制备吸烟诱导的慢性支气管炎大鼠模型,研究大鼠血清髓过氧化物酶(MPO)的变化与巨噬细胞炎性蛋白-2(MIP-2)之间的关系,探讨慢性支气管炎气道炎症形成的可能机制。方法雄性Wistar大鼠随机分为二组:正常对照组、吸烟模型组。采用单纯吸烟的方法建立慢性支气管炎大鼠模型。光镜下观察支气管肺组织病理形态学改变。分析支气管肺泡灌洗液(BALF)细胞计数和分类;用ELISA法测定肺组织匀浆MIP-2质量浓度;用生化比色法测定大鼠血清MPO含量。结果模型组病理形态学改变符合人类慢性支气管炎的特点。与正常组比较,模型组血清MPO及肺组织匀浆MIP-2含量明显升高(P<0.01),模型组血清MPO与BALF中性粒细胞数,肺组织匀浆MIP-2质量浓度成显著正相关(分别为r=0.876及r=0.739;均P<0.01)。结论吸烟诱导的慢性支气管炎大鼠可能通过MIP-2介导中性粒细胞聚集,活化参与气道炎症反应。

小檗碱和大黄酸对LPS诱导巨噬细胞炎症反应及TLR2/NF-κB信号通路的影响

目的观察小檗碱和大黄酸对脂多糖(LPS)诱导巨噬细胞炎症反应及炎性相关信号通路Toll样受体2(TLR2)/核转录因子κB(NF-κB)的影响。方法将巨噬细胞RAW264. 7随机分为4组,空白组以完全培养基常规培养,LPS诱导组加入10 ng/m L LPS诱导4 h,小檗碱组和大黄酸组分别用20μmol/L小檗碱和30μmol/L大黄酸预处理2 h后加入10 ng/m L LPS诱导4 h。ELISA法检测细胞上清液炎性因子IL-1β、IL-6水平,RT-qPCR和Western blotting法分别检测细胞中的TLR2、白细胞介素4受体相关激酶(IRAK4)、NF-κΒp65 mRNA和蛋白。结果与空白组比较,LPS诱导组、小檗碱组和大黄酸组细胞上清液IL-1β、IL-6水平升高(P均<0. 05),细胞中TLR2、IRAK4及NF-κΒp65 mRNA和蛋白表达增加(P均<0. 05);与LPS诱导组比较,小檗碱组和大黄酸组细胞上清液IL-1β、IL-6水平降低(P均<0. 05),细胞中TLR2、NF-κΒp65 mRNA和蛋白及IRAK4 mRNA表达下降(P均<0. 05),小檗碱组IRAK4蛋白表达下降(P <0. 05)。结论小檗碱和大黄酸可通过下调TLR2/NF-κB信号通路分子的表达,从而抑制LPS诱导巨噬细胞炎性因子的产生和释放,以发挥其抗炎作用。

MIP-2、MIP-1α和IL-6在小鼠血流感染中的变化规律实验研究

目的探讨巨噬细胞炎性蛋白2(macrophage inflammatory protein-2,MIP-2)、巨噬细胞炎性蛋白1α(macrophage inflammatory protein-1 Alpha,MIP-1α)和白细胞介素6(interleukin-6,IL-6)在金黄色葡萄球菌和大肠埃希菌感染时的变化规律及在鉴别诊断金黄色葡萄球菌和大肠埃希菌感染的价值。方法将216只ICR小鼠随机分为3组,各组72只。尾静脉注射大肠埃希菌和金黄色葡萄球菌建立小鼠血流感染模型,生理盐水注射建立阴性对照。共9个时间点,各时间点每组8只小鼠。分别在感染0.5 h、1 h、3 h、6 h、12 h、1 d、2 d、3 d、5 d后采血,检测血液白细胞计数(WBC),血清中MIP-2、MIP-1α和IL-6浓度。结果 1大肠埃希菌组和金黄色葡萄球菌组小鼠在感染0.5 h后MIP-2、MIP-1α和IL-6均明显升高,各指标峰值分别为(13 246.8±865.37)pg/ml、(699.79±36.36)pg/ml、(25 080.32±1 263.58)pg/ml、(3 483.22±169.84)pg/ml和(1 171.98±104.49)pg/ml、(94.71±14.38)pg/ml,大肠埃希菌感染组显著高于金黄色葡萄球菌感染组;2MIP-2、MIP-1α和IL-6在大肠埃希菌感染时的ROC曲线下面积(0.962、0.967、0.962)与金黄色葡萄球菌感染时的(0.877、0.889、0.885)的差异有统计学意义(P<0.05),并且两组之间差异也有统计学意义(P<0.05)。结论 MIP-2、MIP-1α和IL-6在炎症早期明显升高,在鉴别大肠埃希菌和金黄色葡萄球菌引发的感染均具有统计学意义。

丙酮酸乙酯对内毒素性急性肺损伤大鼠肺组织巨噬细胞炎症蛋白-2表达的影响

目的观察丙酮酸乙酯（EP）预先给药对内毒素性急性肺损伤（ALI）大鼠肺组织巨噬细胞炎症蛋白-2表达的影响，探讨丙酮酸乙酯可能的保护机制。方法静脉注射脂多糖（LPS）5mg／kg，复制大鼠ALI模型。雄性SD大鼠30只随机分为三组：A组为对照组，B组为LPS组，C组为EP＋LPS组，于静脉注射LPS前1h腹腔内注射EP（40mg／kg）。所有动物于注射LPS或生理盐水后6h颈动脉放血处死，RT-PCR法测定肺组织巨噬细胞炎症蛋白-2mRNA的表达；酶联免疫吸附法测定肺组织TNF-α和IL-1β的含量。结果与A组相比，B组、C组肺组织巨噬细胞炎症蛋白-2mRNA表达增加，肺组织TNF-α和IL-1β含量上升（P〈0．05）；与B组相比，C组肺组织巨噬细胞炎症蛋白-2mRNA表达降低，肺组织TNF-α和IL-1β含量降低（P〈0．05）。结论丙酮酸乙酯通过下调大鼠LPS诱导的肺组织巨噬细胞炎症蛋白-2表达，降低了TNF-α和IL-1β的释放，减轻ALI大鼠肺部的炎症反应。

白藜芦醇对牙髓卟啉单胞菌脂多糖诱导成骨细胞产生MIP-2的影响

目的:研究牙髓卟啉单胞菌(Porphyromonas endodontalis,P.e)脂多糖(lipopolysaccharide,LPS)影响成骨细胞产生巨噬细胞炎性蛋白2(macrophage inflammatory protein-2,MIP-2)mRNA和蛋白分泌的作用,以及白藜芦醇对P.eLPS诱导分泌MIP-2产生的抑制作用。方法:以不同剂量的P.e-LPS (0～50 mg/L)作用于MC3T3-El细胞,并以20 mg/L P.e-LPS作用MC3T3-El细胞不同时间(0～48 h),采用实时反转录PCR (real-time RT-PCR)和酶联免疫吸附试验(ELISA)检测MIP-2 mRNA和蛋白的表达;采用ELISA方法检测白藜芦醇对20 mg/L P.e-LPS刺激MC3T3-El细胞24 h后MIP-2蛋白表达的影响。采用SPSS 13.0软件包对结果进行单因素方差分析和Dunnett t检验。结果:当不同剂量P.e-LPS (0～50 mg/L)刺激MC3T3-El细胞时,MIP-2 mRNA的表达和蛋白的分泌随剂量的提高而升高;其中,蛋白表达从(41.86±2.49)ng/L升高到(3126.74±158.30)ng/L,差异显著(P<0.05)。在观察时间内(0～48 h),20 mg/L P.e-LPS刺激MC3T3-El细胞后,MIP-2 mRNA的表达和蛋白的分泌随时间的延长而增高,48 h时蛋白表达量最高,为(2102.55±123.27)ng/L(P<0.01)。10 mol/L白藜芦醇预处理细胞1 h,可抑制P.e-LPS诱导的MIP-2蛋白的表达,蛋白水平从(1805.33±67.54)ng/L降低到(813.82±47.21)ng/L,差异显著(P<0.01)。结论:P.e-LPS可诱导成骨细胞表达和分泌MIP-2,白藜芦醇对P.e-LPS诱导的MIP-2蛋白分泌发挥抑制作用。