Effects of interleukin-10 treated macrophages on bone marrow mesenchymal stem cells via signal transducer and activator of transcription 3 pathway

BACKGROUND Alveolar bone defects caused by inflammation are an urgent issue in oral implant surgery that must be solved.Regulating the various phenotypes of macrophages to enhance the inflammatory environment can significantly affect the progression of diseases and tissue engineering repair process.AIM To assess the influence of interleukin-10(IL-10)on the osteogenic differentiation of bone marrow mesenchymal stem cells(BMSCs)following their interaction with macrophages in an inflammatory environment.METHODS IL-10 modulates the differentiation of peritoneal macrophages in Wistar rats in an inflammatory environment.In this study,we investigated its impact on the proliferation,migration,and osteogenesis of BMSCs.The expression levels of signal transducer and activator of transcription 3(STAT3)and its activated form,phos-phorylated-STAT3,were examined in IL-10-stimulated macrophages.Subsequently,a specific STAT3 signaling inhibitor was used to impede STAT3 signal activation to further investigate the role of STAT3 signaling.RESULTS IL-10-stimulated macrophages underwent polarization to the M2 type through substitution,and these M2 macrophages actively facilitated the osteogenic differentiation of BMSCs.Mechanistically,STAT3 signaling plays a crucial role in the process by which IL-10 influences macrophages.Specifically,IL-10 stimulated the activation of the STAT3 signaling pathway and reduced the macrophage inflammatory response,as evidenced by its diminished impact on the osteogenic differentiation of BMSCs.CONCLUSION Stimulating macrophages with IL-10 proved effective in improving the inflammatory environment and promoting the osteogenic differentiation of BMSCs.The IL-10/STAT3 signaling pathway has emerged as a key regulator in the macrophage-mediated control of BMSCs’osteogenic differentiation.

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.

Suppression of Breast Cancer Proliferation and Induction of Apoptosis via AKT and ERK1/2 Signal Transduction Pathways by Synthetic Polypeptide Derived from Viral Macrophage Inflammatory Protein Ⅱ

SDF-1α,a ligand for the chemokine receptor CXCR4,is well known for mediating the migration of breast cancer cells.In a previous study we demonstrated that a synthetic 21-mer peptide antagonist of CXCR4（NT21MP） derived from the viral macrophage inflammatory protein Ⅱ could antagonize tumor growth in vivo by inhibiting cellular proliferation and inducing apoptosis in breast cancer cells.However,the role of SDF-1α in the signaling pathways underlying the proliferation of human breast cancer cells and associated signaling pathways and inhibiting signal pathways of NT21MP remained unclear.The present study investigated the mechanism of NT21MP on anti-tumor in breast cancer in vitro.The effect of NT21MP on the viability of cells was determined by the MTT assay.Annexin V-FITC and PI staining was performed to detect early stage apoptosisin SKBR3 cells treated with SDF-1α and AMD3100 or NT21MP.Western blotting techniques were used to assay the composition of phosphoproteomics and total proteins present in the SKBR3 breast cancer cells.RT-PCR and Western blotting technique were used to detect the effect of NT21MP and AMD3100 on Bcl-2 and Bax expression.The results indicated that SDF-1α prevented apoptosis and promoted the proliferation of SKBR3 human breast cancer cells.As compared with untreated SKBR3 cells,Treatment with SDF-1α significantly increased cell viability,and NT21MP abolished the protective effects of SDF-1α dose-dependently（P0.05）.There was a significant decrease in the percentage of apoptotic cells after SDF-1α treatment as compared with control group（2.7%±0.2% vs.5.7%±0.4%,P0.05）.But pretreatment of SKBR3 cells with NT21MP significantly attenuated the antiapoptotic effects of SDF-1α as compared with SKBR3 cells without NT21MP pretreatment.The proliferative and anti-apoptotic effects of SDF-1α in SKBR3 cells were associated with an increase in AKT and ERK1/2 phosphorylation as well as a decrease in Bax expression and an increase in Bcl-2 expression.These changes in intracellular processes were blocked by NT21MP in a dose-dependent manner（P0.05）.In conclusion,NT21MP efficiently inhibits SDF-1α-induced proliferation and antiapoptosis in SKBR3 cells by reducing the levels of phosphorylated AKT and ERK1/2,as well as decreasing the ratio of expression of Bcl-2 relative to Bax.

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.

Expression of macrophage inflammatory protein-1αin Kupffer cells following liver ischemia or reperfusion injury in rats

瞄准：探索巨噬细胞的表示在在老鼠跟随肝 ischemia/reperfusion 损害 IRI 的 Kupffer 房间(KC ) 的煽动性的 protein-1alpha (MIP-1alpha ) 。方法：四十只男 SD 老鼠随机被划分成五个组。在老鼠肝的部分温暖的 ischemia/reperfusion 损害的一个模型被建立。KC 在灌注以后被孤立并且孵化一个小时，六个小时， 12 h，和 24 h。肿瘤坏死因素高山哈(TNF-alpha ) 并且在上层清液的 interleukin-1beta (IL-1beta ) 被 ELISA 测量。在 KC 的 MIP-1alpha 被细胞化学的免疫和 RT-PCR 检测。结果：没有或很少 MIP-1alpha 蛋白质和 mRNA 在控制组的 KC 被表示。它在 IRI 组的表达式在灌注以后有重要增加(P 【 0.05 ) ，它与控制组相反。结论：在 KC 后面的肝 ischemia/reperfusion 损害的 MIP-1alpha 基因的活跃行为被假定是为肝的 ischemia/reperfusion 损害的主要原因之一。

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.

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.

NLRP3炎性小体在治疗性浅低温后处理大鼠心肌缺血-再灌注中的作用

目的 分析NOD样受体热蛋白结构域相关蛋白3(NLRP3)炎性小体在治疗性浅低温(34℃)后处理的大鼠离体心肌缺血-再灌注模型中的作用并探讨其机制。方法 选择清洁级成年雄性SD大鼠60只,7~10周龄,体重250~300 g。采用随机数字表法将大鼠分为五组:空白对照组(S组)、心肌缺血-再灌注组(IR组)、34℃浅低温后处理心肌缺血-再灌注组(MH组)、34℃浅低温后处理心肌缺血-再灌注+3-TYP组(HT组)和34℃浅低温后处理心肌缺血-再灌注+3-TYP+MCC950组(HTM组),每组12只。S组在37℃灌流液平衡灌流大鼠心脏180 min;IR组在37℃灌流液平衡灌流大鼠心脏30 min后,缺血30 min, 37℃灌注液再灌注120 min;MH组在37℃灌流液平衡灌流大鼠心脏30 min后,缺血30 min, 34℃灌注液再灌注120 min;HT组在37℃灌流液平衡灌流大鼠心脏30 min后,缺血30 min,在灌注液中加入沉默信息调节因子2同源蛋白3(sirt3)抑制剂3-TYP后行34℃灌注液再灌注120 min;HTM组在37℃灌流液平衡灌流大鼠心脏30 min后,缺血30 min,在灌注液中加入sirt3抑制剂3-TYP和NLRP3抑制剂MCC950后行34℃灌注液再灌注120 min。再灌注120 min后取离体心脏,采用ELISA法测定灌注后心脏漏液中IL-1β、IL-6浓度,Western blot法检测心肌组织中NLRP3和sirt3蛋白相对含量,1%氯化三苯基四氮唑染色计算心肌梗死面积,HE染色观察心肌病理变化。结果 与S组比较,IR组、MH组、HT组和HTM组再灌注30、60、90、120 min时HR明显减慢,LVSP、dp/dt_(max)明显降低,LVEDP明显升高;心脏漏液中IL-6和IL-1β浓度、心肌梗死面积百分比明显升高(P<0.05);IR组、HT组和HTM组心肌组织中sirt3蛋白含量明显降低,NLRP3蛋白含量明显升高(P<0.05);MH组心肌组织中sirt3和NLRP3蛋白含量明显升高(P<0.05)。与IR组比较,MH组和HTM组再灌注30、60、90、120 min时HR明显增快,LVSP、±dp/dt_(max)明显升高,LVEDP明显降低;心脏漏液中IL-6和IL-1β浓度、心肌梗死面积百分比明显降低(P<0.05);MH组心肌组织中sirt3蛋白含量明显升高,NLRP3蛋白含量明显降低(P<0.05);HTM组心肌组织中NLRP3蛋白含量明显降低(P<0.05)。与MH组比较,HT组再灌注30、60、90、120 min时HR明显减慢,LVSP、±dp/dt_(max)明显降低,LVEDP明显升高;心脏漏液中IL-6和IL-1β浓度、心肌梗死面积百分比、心肌组织中NLRP3蛋白含量明显升高(P<0.05);HT组和HTM组心肌组织中sirt3蛋白含量明显降低(P<0.05)。与HT组比较,HTM组再灌注30、60、90、120 min时HR明显增快,LVSP、±dp/dt_(max)明显升高,LVEDP明显降低;心脏漏液中IL-6和IL-1β浓度、心肌梗死面积百分比、心肌组织中NLRP3蛋白含量明显降低(P<0.05)。结论 治疗性浅低温(34℃)可通过改善离体心脏血流动力学参数、降低IL-6、IL-1β浓度、心肌组织中NLRP3蛋白含量、心肌梗死面积百分比、改善心肌病理学改变,减轻大鼠心肌缺血-再灌注损伤,其机制可能与线粒体介导sirt3通路抑制炎性小体NLRP3的高表达有关。

急性脑梗死患者血清miR-22-3p、NLRP3水平与炎性因子及预后不良的关系

目的探讨急性脑梗死(ACI)患者血清微小核糖核酸-22-3p(miR-22-3p)、NOD样受体热蛋白结构域相关蛋白3(NLRP3)水平与炎性因子及预后不良的关系。方法选取2021年1月—2022年12月上海中医药大学附属第七人民医院神经内科收治ACI患者106例为ACI组,根据预后情况分为预后不良亚组37例和预后良好亚组69例,另选取同期体检健康者60例为健康对照组。采用实时荧光定量聚合酶链式反应检测血清miR-22-3p水平,酶联免疫吸附法检测血清NLRP3和炎性因子[白介素(IL)-1β、IL-18、肿瘤坏死因子-α(TNF-α)]水平。通过Pearson相关性分析ACI患者血清miR-22-3p、NLRP3与IL-1β、IL-18、TNF-α的相关性。分析ACI患者预后不良的影响因素,绘制2项指标的受试者工作特征(ROC)曲线分析其预测预后的价值。结果与健康对照组比较,ACI组血清miR-22-3p水平降低,NLRP3、IL-1β、IL-18、TNF-α水平显著升高(t/P=18.698/<0.001、27.091/<0.001、30.154/<0.001、35.104/<0.001、39.834/<0.001)。Pearson相关性分析显示,ACI患者血清miR-22-3p与NLRP3、IL-1β、IL-18、TNF-α水平呈负相关(r/P=-0.733/<0.001、-0.719/<0.001、-0.683/<0.001、-0.680/<0.001),血清NLRP3与IL-1β、IL-18、TNF-α水平呈正相关(r/P=0.716/<0.001、0.715/<0.001、0.707/<0.001)。多因素Logistic回归分析显示,NIHSS评分、IL-1β、IL-18、TNF-α、NLRP3升高为ACI患者预后不良的独立危险因素[OR(95%CI)=1.244(1.034~1.497)、1.373(1.067~1.767)、1.047(1.011~1.086)、1.577(1.061~2.343)、1.084(1.022~1.149)],miR-22-3p升高为独立保护因素[OR(95%CI)=0.933(0.888~0.980)]。ROC曲线分析显示,血清miR-22-3p、NLRP3水平联合预测ACI患者预后不良的曲线下面积为0.875,大于两者单独预测的0.786、0.759(Z/P=2.405/0.016、2.517/0.012)。结论ACI患者血清miR-22-3p水平降低和NLRP3水平升高,与炎性因子水平升高和预后不良密切相关,血清miR-22-3p、NLRP3水平联合对ACI患者预后不良的预测价值较高。

急性呼吸窘迫综合征患儿血清Melatonin、MIP-1α与NLRP3炎症小体和预后的关系分析

目的探讨急性呼吸窘迫综合征(ARDS)患儿血清褪黑素(Melatonin)、巨噬细胞炎性蛋白-1α(MIP-1α)与核苷酸结合寡聚化结构域样受体蛋白3(NLRP3)炎症小体和预后的关系。方法选取2021年1月至2023年1月该院收治的ARDS患儿140例纳入ARDS组,另选取同期100例体检健康儿童纳入对照组。根据入院28 d临床结局将ARDS患儿分为死亡组29例和存活组111例。采用酶联免疫吸附试验检测血清Melatonin、MIP-1α、白细胞介素(IL)-1β、IL-18水平,实时荧光定量PCR检测NLRP3 mRNA、半胱氨酸蛋白酶-1(Caspase-1)mRNA水平。采用Pearson相关分析ARDS患儿血清Melatonin、MIP-1α水平与NLRP3炎症小体相关指标(NLRP3 mRNA、Caspase-1 mRNA、IL-1β、IL-18)的相关性。采用多因素Cox回归分析影响ARDS患儿预后的因素。根据ARDS患儿血清Melatonin、MIP-1α水平均值分为高/低血清Melatonin、MIP-1α组,Kaplan-Meier法绘制高/低血清Melatonin、MIP-1α水平ARDS患儿生存曲线。采用受试者工作特征(ROC)曲线分析血清Melatonin、MIP-1α对ARDS患儿死亡的预测价值。结果与对照组比较,ARDS组血清Melatonin水平降低,血清MIP-1α、IL-1β、IL-18和外周血单核细胞NLRP3 mRNA、Caspase-1 mRNA水平升高(P<0.05)。Pearson相关分析显示,ARDS患儿血清Melatonin水平与NLRP3 mRNA、Caspase-1 mRNA、IL-1β、IL-18均呈负相关(P<0.05),MIP-1α水平与NLRP3 mRNA、Caspase-1 mRNA、IL-1β、IL-18均呈正相关(P<0.05)。多因素Cox回归分析显示,急性生理学和慢性健康状况评价Ⅱ评分、NLRP3 mRNA、Caspase-1 mRNA、IL-1β、IL-18、MIP-1α为影响ARDS患儿预后的独立危险因素,Melatonin为独立保护因素(P<0.05)。Kaplan-Meier生存曲线分析显示,高血清Melatonin组28 d生存率高于低血清Melatonin组(P<0.05),高血清MIP-1α组28 d生存率低于低血清MIP-1α组(P<0.05)。ROC曲线分析显示,血清Melatonin、MIP-1α联合预测ARDS患儿死亡的曲线下面积为0.881(95%CI 0.816~0.930),大于血清Melatonin、MIP-1α单独预测的0.785(95%CI 0.708~0.850)、0.778(95%CI 0.700~0.844)。结论ARDS患儿血清Melatonin水平降低、MIP-1α水平升高,与NLRP3炎症小体和预后密切相关,联合检测血清Melatonin、MIP-1α水平对ARDS患儿预后具有较高的预测价值。

血清COL10A1、TK1、MIP-3α水平与胃癌患者病理特征的关系及其对腹膜转移的诊断价值研究

目的研究血清X型胶原α1链(COL10A1)、胸苷激酶1(TK1)、巨噬细胞炎症蛋白-3α(MIP-3α)水平与胃癌患者病理特征的关系及其对胃癌腹膜转移的诊断价值。方法以2021年1月至2022年12月邢台市人民医院收治的96例胃癌患者作为恶性组,其中有腹膜转移27例,无腹膜转移69例;选取同期收治的104例胃良性病变患者作为良性病变组,选取112例健康体检者作为健康对照组。比较各组血清COL10A1、TK1、MIP-3α水平及不同病理特征、有无腹膜转移胃癌患者血清COL10A1、TK1、MIP-3α水平,采用受试者工作特征(ROC)曲线分析血清COL10A1、TK1、MIP-3α对胃癌患者腹膜转移的诊断价值。结果恶性组血清COL10A1、MIP-3α、TK1水平高于健康对照组、良性病变组,良性病变组血清COL10A1、MIP-3α水平高于健康对照组,差异均有统计学意义(P<0.05)。低/未分化、有脉管浸润、肿瘤临床病理分期(TNM)分期Ⅲ~Ⅳ期胃癌患者血清COL10A1、TK1、MIP-3α水平高于高/中分化、无脉管浸润、TNM分期Ⅰ~Ⅱ期患者(P<0.05)。有腹膜转移胃癌患者血清COL10A1、TK1、MIP-3α水平高于无腹膜转移患者(P<0.05)。血清COL10A1、TK1、MIP-3α单项及3项联合检测诊断胃癌腹膜转移的曲线下面积(AUC)分别为0.722(95%CI:0.621~0.809)、0.749(95%CI:0.651~0.832)、0.736(95%CI:0.637~0.821)、0.853(95%CI:0.766~0.917),3项联合检测诊断的AUC大于3项单独检测(Z=1.990、3.617、2.986,P<0.001)。结论胃癌的发生导致患者血清COL10A1、TK1、MIP-3α水平升高,同时随着胃癌患者病情的进展,血清COL10A1、TK1、MIP-3α水平升高,且3项指标联合检测对胃癌患者腹膜转移具有较好的诊断价值。

NLRP3炎症小体参与糖尿病肾病肾间质纤维化机制的研究进展

肾间质纤维化(RIF)是糖尿病肾病(DN)进展至终末期肾病的不可逆因素。慢性炎症是DN-RIF发病机制的关键原因,NOD样受体热蛋白结构域相关蛋白3(NLRP3)炎症小体作为重要的炎症调节因子,可通过炎症反应、氧化应激、自噬等机制促进DN-RIF的发生。本文对NLRP3炎症小体与RIF发生发展的机制及传统中药针对NLRP3炎症小体为靶点对RIF的治疗作用作一综述,以期对未来治疗RIF提供帮助。

EGR3通过抑制PRMT1/p-STAT3通路减轻肥胖相关性肾病足细胞炎症损伤

目的:肥胖会导致肥胖相关性肾病(obesity related glomerulopathy,ORG),但其发病机制并不明确。本研究拟检测早期生长反应蛋白3(early growth response protein 3,EGR3)在ORG患者和高脂饮食诱导的肥胖小鼠肾皮质组织中的表达,并探讨EGR3抑制棕榈酸(palmitic acid,PA)诱导的人足细胞炎症损伤的分子机制。方法:收集排除其他疾病导致的肾损害并经组织病理学证实的ORG患者(n=6)和高脂饮食诱导的肥胖小鼠的肾皮质组织(n=10)。使用150μmol/L PA干预人和小鼠足细胞48 h;人足细胞中分别过表达或沉默EGR3。采用酶联免疫吸附试验(enzyme linked immunosorbent assay,ELISA)检测白细胞介素(interleukin,IL)-6和IL-1β的含量;real-time RT-PCR检测EGR3、足细胞分子标志NPHS1(nephrosis1)、NPHS2(nephrosis2)、足糖萼蛋白(podocalyxin,PODXL)、平足蛋白(podoplanin,PDPN)mRNA的表达;RNA-seq检测人足细胞过表达EGR3并150μmol/L PA干预后与对照组的差异表达基因(differentially expressed genes,DEGs);免疫共沉淀(co-immunoprecipitation,Co-IP)+液相色谱串联质谱(liquid chromatography tandem mass spectrometry,LC-MS)检测EGR3可能的相互作用蛋白质,并与RNA-seq的结果取交集;Co-IP验证EGR3与蛋白精氨酸甲基转移酶1(protein arginine methyltransferases 1,PRMT1)的相互作用;沉默EGR3和PRMT1抑制剂干预后检测PA诱导的足细胞培养液中IL-6和IL-1β的含量;蛋白质印迹法检测分别过表达或沉默EGR3后磷酸化信号转导及转录激活蛋白3(phosphorylated signal transducer and activator of transcription 3,p-STAT3)的蛋白质表达。结果:EGR3在ORG患者和高脂饮食诱导的肥胖小鼠肾皮质组织中的表达均显著上调(均P<0.01),150μmol/L PA干预人和小鼠足细胞48 h后显著上调2种细胞EGR3的表达(均P<0.05)。人足细胞过表达或沉默EGR3分别抑制或促进PA干预后细胞培养液中IL-6和IL-1β的分泌,并分别上调或下调NPHS1、PODXL、NPHS2及PDPN的表达(均P<0.05)。RNA-seq结果显示共有988个DEGs,Co-IP+LC-MS共发现238个可能与EGR3相互作用的蛋白质,且Co-IP证实PRMT1为EGR3的相互作用蛋白质。PRMT1抑制剂能部分减少人足细胞沉默EGR3后PA诱导的IL-6及IL-1β的分泌(均P<0.05);此外,过表达或沉默EGR3负调控PRMT1及p-STAT3的表达。结论:EGR3可能通过抑制PRMT1/p-STAT3通路减轻ORG足细胞炎症损伤。

电针抑制NLRP3炎性小体活化改善缺血性脑卒中的机制研究

目的观察电针对缺血性脑卒中大鼠神经行为学及脑组织结构的影响,探讨电针通过调控NOD样受体热蛋白结构域相关蛋白3(NOD-like receptor thermal protein domain associated protein 3,NLRP3)炎性小体途径改善缺血性脑卒中大鼠神经功能的机制。方法36只健康雄性SD大鼠采用随机数字表随机分为假手术组12只及手术组24只,手术组大鼠采用Longa等改良线栓法制备大鼠脑缺血再灌注损伤(MCAO)模型。术后2 h行神经行为学评分,造模成功的大鼠再随机分为模型组及电针组。电针组予电针“曲池”“足三里”连续干预7 d,假手术组及模型组不做干预。干预完成后分别评估各组大鼠神经功能缺损情况,HE染色观察脑组织病理学变化,QPCR及Western blot法检测炎性小体相关蛋白NLRP3、ASC、Caspase-1的表达水平,ELISA检测各组大鼠血清IL-1β和IL-18炎性因子表达。结果与假手术组相比,模型组大鼠神经功能评分均显著提高,差异有高度统计学意义(P<0.01),脑组织缺血皮质区神经元胞体缩小变形,核固缩明显,大鼠脑组织缺血周围区炎性因子相关蛋白NLRP3、ASC、Caspase-1的mRNA及蛋白表达水平升高,差异有高度统计学意义(P<0.01),血清IL-1β和IL-18炎症因子表达增加,差异有高度统计学意义(P<0.01);经电针干预7 d后,电针组神经评分功能较模型组显著下降,差异有统计学意义(P<0.05),所见的病理损伤减少;炎性小体相关蛋白NLRP3、ASC、Caspase-1的表达下降,差异有统计学意义(P<0.05),且电针下调了血清IL-1β和IL-18的表达,差异有统计学意义(P<0.05)。结论电针“曲池”“足三里”可减轻缺血性脑卒中大鼠神经功能缺损症状,减少脑组织病理损伤,下调NLRP3、ASC、Caspase-1表达水平,其机制可能与调控NLRP3炎性小体途径抗细胞焦亡,减轻脑缺血再灌注损伤有关。

急性脑梗死患者外周血炎性小体NLRP3表达及与颅内动脉血栓病理成分、预后的相关性分析

目的 探讨急性脑梗死(ACI)患者外周血炎性小体NOD样受体热蛋白结构域相关蛋白3(NLRP3)表达,并分析其与颅内动脉血栓病理成分、预后的相关性。方法 选取2022年1—12月收治的92例ACI作为观察组,另选取健康志愿者92例作为对照组,检测外周血NLRP3 mRNA、蛋白及血清水平。观察组行机械取栓治疗,采用HE染色法半定量分析血栓取出物,并分为红细胞富集血栓者、纤维蛋白富集血栓者。比较不同组别、不同血栓病理成分、不同预后患者外周血炎性小体NLRP3水平,分析其与血栓病理成分相关性及对预后不良风险的关系。结果 观察组NLRP3 mRNA、蛋白表达及血清水平高于对照组,红细胞富集血栓者高于纤维蛋白富集血栓者,且与红细胞富集血栓呈正相关(P<0.05,P<0.01);预后不良者NLRP3 mRNA、蛋白表达及血清水平高于预后良好者(P<0.01);NLRP3 mRNA、蛋白高表达及血清高水平患者预后不良风险分别是低表达、低水平患者的2.182、2.500、2.182倍(P<0.05)。结论 ACI患者外周血炎性小体NLRP3水平升高,且与颅内动脉红细胞富集血栓相关,可增加预后不良发生风险。

抗炎通腑方对脓毒症急性肺损伤大鼠mtDNA-STING-NLRP3信号通路的影响

目的探讨抗炎通腑方对脓毒症急性肺损伤(ALI)大鼠的影响及作用机制。方法将35只大鼠随机分为正常组、模型组、地塞米松(DEX)组、中药(TCM)组和TCM+DEX组,每组7只。分别给予相应药物灌胃、造模。酶联免疫吸附实验(ELISA)法检测白细胞介素(IL)-6、IL-1β、IL-18、肿瘤坏死因子-α(TNF-α)含量及血清中巨噬细胞计数;采用实时荧光定量多聚核苷酸链式反应(RT-qPCR)和蛋白免疫印迹(Western blot)检测肺组织中干扰素基因刺激因子(STING)、磷酸化干扰素基因刺激因子(P-STING)、NOD样受体热蛋白结构域相关蛋白3(NLRP3)、凋亡相关斑点样蛋白信使核糖核酸(ASC mRNA)和相关蛋白的表达水平。测定肺组织湿/干比(W/D),观察肺组织病理学改变。检测肺组织中巨噬细胞表达情况。结果与正常组比较,各组指标显著升高;与模型组比较,DEX组、TCM组及TCM+DEX组各指标均显著降低。与模型组比较,TCM+DEX组改变最为明显,肺组织损伤改善,W/D值(4.77±0.29 vs.3.78±0.48)及巨噬细胞计数(13.39±2.06 vs.7.09±1.42)均降低(P<0.05),IL-6(152.51±22.27 vs.58.92±13.53)、IL-1β(126.19±10.02 vs.45.69±6.67)、IL-18(59.12±6.31 vs.31.75±4.23)及TNF-α(126.57±8.25 vs.49.59±8.12)水平均降低(P均<0.01),肺组织中线粒体DNA(mtDNA)损伤及释放、P-STING(0.32±0.03 vs.0.16±0.03)、STING mRNA(19.24±2.70 vs.0.32±0.16)、NLRP3 mRNA(20.03±5.06 vs.1.20±0.04)、ASC mRNA(16.96±4.31 vs.3.41±2.52)和相关蛋白的表达均降低(P<0.01)。结论抗炎通腑方可能通过调控mtDNA-STING-NLRP3信号通路减轻脓毒症ALI大鼠的炎症。

妊娠期胎膜早破患者血清GATA-3及MIP-3Α水平对羊膜腔内感染的诊断价值

目的探讨妊娠期胎膜早破患者血清GATA结合蛋白-3(GATA-3)联合巨噬细胞炎性蛋白-3α(MIP-3α)水平对羊膜腔内感染的诊断价值。方法回顾性分析,选取2021年10月至2023年8月在渭南市中心医院治疗的123例妊娠期胎膜早破患者作为研究对象,将是否发生羊膜腔内感染分为感染组(53例)和未感染组(70例)。感染组年龄(27.65±3.58)岁,孕周(36.47±3.04)周;未感染组年龄(27.71±3.69)岁,孕周(37.52±3.27)周。对比两组患者产前血清GATA-3和MIP-3α水平。受试者工作特征曲线(ROC)评估GATA-3、MIP-3α水平对妊娠期胎膜早破患者发生羊膜腔内感染的诊断价值,多因素logistic回归分析影响妊娠期胎膜早破患者发生羊膜腔内感染的危险因素。统计学方法采用t检验、χ^(2)检验。结果感染组血清GATA-3水平低于未感染组[(261.35±27.87)ng/L比(292.87±29.53)ng/L],MIP-3α水平高于未感染组[(38.84±6.33)μg/L比(29.61±5.62)μg/L],差异均有统计学意义(t=6.005、8.540,均P<0.05)。GATA-3、MIP-3α预测胎膜早破合并羊膜腔内感染的曲线下面积(AUC)分别为0.789、0.855,截断值分别为276.74 ng/L、36.04μg/L,特异度分别为77.4%、88.6%,灵敏度分别为75.7%、71.7%,二者联合检测的AUC为0.924,特异度为94.3%,灵敏度为81.1%。GATA-3≤276.74 ng/L、MIP-3α≥36.04μg/L、有流产及引产史、未足月胎膜早破是妊娠期胎膜早破患者发生羊膜腔内感染的独立风险因素(均P<0.05)。结论血清GATA-3、MIP-3α水平异常是影响胎膜早破患者并发羊膜腔内感染的危险因素,对于羊膜腔内感染的诊断具有较高价值。

TLR4/NF-κB/NLRP3通路抑制炎症反应作用的研究

Toll样受体(TLRs)是参与非特异性免疫的一类重要的蛋白质,是表达与固有免疫细胞最重要的模式识别受体之一,可识别来源于微生物的具有保守结构的分子,即病原体相关分子模式(PAMAs),从而激活机体产生免疫应答。核因子κB(NF-κB)在几乎所有类型的细胞和组织中都有表达,在调节对外部刺激的显著多样性的反应中起着关键作用,因此是多个生理和病理过程中的关键因素。而核苷酸结合寡聚化结构域样受体蛋白3(NLRP3),即NLRP3炎性小体通路在脑缺血再灌注和焦亡中具有重要意义,如NLRP3在脑缺血再灌注损伤时在小胶质细胞中被激活,随后在神经元和微血管内皮细胞中表达。由TLRs激活、NF-κB传递、NLRP3启动形成的TLR/NF-κB/NLRP3信号通路在机体各器官炎症反应中起到关键性作用,本文探讨了各类药物通过抑制该通路炎症反应,起到保护身体各大重要器官的作用。

基于肠道炎症反应研究降糖3号方抗糖尿病的作用机制

目的:观察降糖3号方对2型糖尿病小鼠肠道炎症相关指标的影响,揭示其抗糖尿病的作用机制。方法:选取4周龄C57BL/6N雄性小鼠,高脂饲料联合小剂量链脲佐菌素(STZ)注射构建2型糖尿病小鼠模型,采用随机数字表法将成模小鼠分成模型组、二甲双胍组、降糖3号方组,每组8只。选取8只标准饲料喂养的小鼠作为正常组。药物干预8周结束后,应用细胞因子抗体芯片技术检测小鼠结肠组织中多种炎症介质水平,并进行差异表达蛋白筛选、基因本体(GO)蛋白功能、京都基因和基因组百科全书(KEGG)通路分析。蛋白质印迹法检测各组小鼠结肠组织中核苷酸结合寡聚化结构域样受体蛋白3(NLRP3)炎症小体激活与肠道黏膜屏障相关的因子G蛋白偶联受体43(GPR43)、凋亡相关斑点样蛋白(ASC)、胱天蛋白酶(Caspase-1)以及闭锁小带蛋白-1(ZO-1)、闭合蛋白(Occludin)的蛋白表达水平。结果:各组间肠道炎症介质差异明显,与模型组比较,降糖3号方组IL-1β、IL-6等炎症介质表达下降,降糖3号方可上调结肠组织中ZO-1、Occludin、GPR43蛋白表达水平,降低ASC、Caspase-1蛋白表达水平(P<0.05)。结论:2型糖尿病小鼠结肠炎症反应明显,降糖3号方能够有效抑制2型糖尿病小鼠肠道炎症,其作用可能与调控NLRP3炎症小体,进而影响下游炎症介质有关。

宫颈癌患者淋巴结转移的危险因素分析及血清TFF3、AIF-1、S100-A11、DKK1预测价值分析

目的 探讨宫颈癌患者淋巴结转移的危险因素分析及血清三叶因子3(trefoil factor 3,TFF3)、同种异体移植物炎性因子-1(allograft inflammatory factor-1,AIF-1)、S100钙结合蛋白-A11(S100 calcium-binding protein-A11,S100-A11)、Wnt通路抑制因子Dickkopf-1(Wnt pathway inhibitor Dickkopf-1,DKK1)的预测价值。方法 选择2021年1月—2023年1月本院收治的71例宫颈癌患者作为研究对象,根据患者有无盆腔淋巴结转移分为淋巴结转移阳性组(28例)和淋巴结转移阴性组(43例)两组。收集两组患者临床病理特征,并检测血清TFF3、AIF-1、S100-A11、DKK1水平。结果 单因素分析显示,FIGO分期、宫旁浸润、肌层浸润、血清TFF3、S100-A11、DKK1是患者发生宫颈癌淋巴结转移的影响因素(P<0.05)。与年龄、分化程度、肿瘤大小、组织学类型、脉管浸润及血清AIF-1无关(P>0.05);Logistic多元回归分析显示,FIGO分期、宫旁浸润、肌层浸润及血清TFF3是影响宫颈癌淋巴结转移的独立因素(P<0.05);ROC曲线分析显示,TFF3对淋巴结转移有中等预测价值(AUC=0.649),明显大于机会参考线下面积(P<0.05)。而AIF-1、S100-A11、DKK1对淋巴结转移无预测价值(AUC分别为0.477、0.517、0.524),与机会参考线下面积比较无统计学意义(P>0.05)。结论 FIGO分期高、宫旁浸润、肌层浸润、血清TFF3异常升高是宫颈癌淋巴结转移的危险因素,血清TFF3有望成为预测宫颈癌淋巴结转移的新标志物;血清AIF-1、S100-A11、DKK1对宫颈癌淋巴结转移的预测效能不理想。