Neutrophil peptide 1 accelerates the clearance of degenerative axons during Wallerian degeneration by activating macrophages after peripheral nerve crush injury

Macrophages play an important role in peripheral nerve regeneration,but the specific mechanism of regeneration is still unclear.Our preliminary findings indicated that neutrophil peptide 1 is an innate immune peptide closely involved in peripheral nerve regeneration.However,the mechanism by which neutrophil peptide 1 enhances nerve regeneration remains unclear.This study was designed to investigate the relationship between neutrophil peptide 1 and macrophages in vivo and in vitro in peripheral nerve crush injury.The functions of RAW 264.7 cells we re elucidated by Cell Counting Kit-8 assay,flow cytometry,migration assays,phagocytosis assays,immunohistochemistry and enzyme-linked immunosorbent assay.Axonal debris phagocytosis was observed using the CUBIC(Clear,Unobstructed Brain/Body Imaging Cocktails and Computational analysis)optical clearing technique during Wallerian degeneration.Macrophage inflammatory factor expression in different polarization states was detected using a protein chip.The results showed that neutrophil peptide 1 promoted the prolife ration,migration and phagocytosis of macrophages,and CD206 expression on the surfa ce of macrophages,indicating M2 polarization.The axonal debris clearance rate during Wallerian degeneration was enhanced after neutrophil peptide 1 intervention.Neutrophil peptide 1 also downregulated inflammatory factors interleukin-1α,-6,-12,and tumor necrosis factor-αin invo and in vitro.Thus,the results suggest that neutrophil peptide 1 activates macrophages and accelerates Wallerian degeneration,which may be one mechanism by which neutrophil peptide 1 enhances peripheral nerve regeneration.

Atherosis-associated lnc_000048 activates PKR to enhance STAT1-mediated polarization of THP-1 macrophages to M1 phenotype

Our previous study has demonstrated that lnc_000048 is upregulated in large-artery atherosclerotic stroke and promotes atherosclerosis in ApoE^(-/-)mice.However,little is known about the role of lnc_000048 in classically activated macrophage(M1)polarization.In this study,we established THP-1-derived testing state macrophages(M0),M1 macrophages,and alternately activated macrophages(M2).Real-time fluorescence quantitative PCR was used to verify the expression of marker genes and the expression of lnc_000048 in macrophages.Flow cytometry was used to detect phenotypic proteins(CD11b,CD38,CD80).We generated cell lines with lentivirus-mediated upregulation or downregulation of lnc_000048.Flow cytometry,western blot,and real-time fluorescence quantitative PCR results showed that down-regulation of lnc_000048 reduced M1 macrophage polarization and the inflammation response,while over-expression of lnc_000048 led to the opposite effect.Western blot results indicated that lnc_000048 enhanced the activation of the STAT1 pathway and mediated the M1 macrophage polarization.Moreover,catRAPID prediction,RNA-pull down,and mass spectrometry were used to identify and screen the protein kinase RNA-activated(PKR),then catRAPID and RPIseq were used to predict the binding ability of lnc_000048 to PKR.Immunofluorescence(IF)-RNA fluorescence in situ hybridization(FISH)double labeling was performed to verify the subcellular colocalization of lnc_000048 and PKR in the cytoplasm of M1 macrophage.We speculate that lnc_000048 may form stem-loop structure-specific binding and activate PKR by inducing its phosphorylation,leading to activation of STAT1 phosphorylation and thereby enhancing STAT1 pathway-mediated polarization of THP-1 macrophages to M1 and inflammatory factor expression.Taken together,these results reveal that the lnc_000048/PKR/STAT1 axis plays a crucial role in the polarization of M1 macrophages and may be a novel therapeutic target for atherosclerosis alleviation in stroke.

三黄糖肾康颗粒治疗糖尿病肾病患者的疗效观察及对TLR4、NF-κB、MCP-1的影响

目的:观察三黄糖肾康颗粒治疗糖尿病肾病的疗效及对血清Toll样受体4(TLR4)、核转录因子-kB(NF-κB)、人单核细胞趋化蛋白-1(MCP-1)的影响。方法:60例DN患者,随机分为观察组和对照组各30例。两组均予以西医基础治疗,观察组在对照组治疗基础上加用三黄糖肾康颗粒,两组疗程均为12周;评价疗效,ELISA检测血清TLR4、NF-κB、MCP-1含量。结果:观察组疗效优于对照组(P<0.05);两组治疗后血清TLR4、NF-κB、MCP-1均降低(P<0.05);与对照组比较,观察组TLR4、NF-κB、MCP-1降低更明显(P<0.05)。两组不良反应发生率差异无统计学意义(P>0.05)。结论:三黄糖肾康颗粒可提高西医常规治疗DN的疗效,调节TLR4、NF-κB、MCP-1水平是其部分作用机制。

MCP-1基因对脓毒症急性肾损伤发生的作用研究

目的研究单核细胞趋化蛋白-1(MCP-1)基因对脓毒症急性肾损伤(AKI)发生的作用。方法选取2022年9月-2023年9月新疆维吾尔自治区人民医院重症医学科收治的50例脓毒症AKI患者作为AKI组,纳入同期50例健康受试者作为对照组。分别采集全部受试者清晨空腹静脉血5 mL,采用ELISA法测定AKI患者及健康人群血清中MCP-1的表达情况;通过原代培养肾小管上皮细胞,利用CK14和CK18抗体进行细胞免疫荧光鉴定,过表达和干扰MCP-1基因,利用CCK8细胞增殖检测试剂盒和RT-qPCR检测肾小管上皮细胞增殖情况和肿瘤坏死因子α(TNF-α)、白细胞介素-1β(IL-1β)、白细胞介素6(IL-6)、白细胞介素10(IL-10)、γ-干扰素(IFN-γ)炎性因子表达的变化。结果与对照组相比,AKI组患者外周血中和尿液中的MCP-1表达量显著升高(P均<0.05);通过细胞免疫荧光鉴定,选择上皮细胞标志物CK14和CK18,原代培养24 h,90%以上的细胞表达细胞标志物CK18,约84%的细胞表达CK14;与NC组相比,siRNA组在24、48 h细胞数量增加(P均<0.05);与MCP-1组相比,siRNA组在24、48、72 h的细胞数量增加(P均<0.05);NC组的IL-1β、IL-6、INF-γ因子的表达水平随时间推移逐渐升高,MCP-1组的IL-1β、IL-6、IL-10、INF-γ和TNF-α因子的表达水平随时间推移逐渐升高,siRNA组的IL-1β、IL-6、INF-γ因子表达水平随时间推移无明显升高趋势。结论MCP-1基因在脓毒症急性肾损伤的发病机制中可能发挥重要作用,该基因可能通过调节IL-1β等炎性细胞因子的表达来抑制肾小管上皮细胞的生长和增殖,从而参与脓毒症患者的AKI过程。

血清ICAM-1 Hcy及MCP-1水平与视网膜静脉阻塞患者血管内皮功能的相关性

目的:探讨血清细胞间黏附因子-1(Intercellular abhesion molecule-1,ICAM-1),同型半胱氨酸(Homocysteine,Hcy)及单核细胞趋化蛋白-1(Monocyte chemotactic protein-1,MCP-1)水平与视网膜静脉阻塞(Retinal vein occlusion,RVO)患者血管内皮功能的相关性。方法:采用回顾性分析我院在2020年7月至2023年10月期间收治的RVO患者95例为RVO组,另选取同期于本院行体检的健康人群102例作为正常对照组。比较两组ICAM-1、Hcy、MCP-1、血管内皮功能[内皮素-1(Endothelin-1,ET-1)、一氧化氮(Nitric oxide,NO)]水平;比较RVO组不同疾病类型ICAM-1、Hcy、MCP-1、ET-1及NO水平;比较不同病情程度ICAM-1、MCP-1、ET-1及NO水平;分析血清ICAM-1、Hcy、MCP-1水平与RVO患者血管内皮功能的相关性。结果:RVO组血清ICAM-1、Hcy、MCP-1、ET-1水平高于对照组,NO水平低于对照组(P<0.05);CRVO患者的血清ICAM-1、Hcy、MCP-1、ET-1水平高于BRVO患者,NO水平低于BRVO患者(P<0.05);ICAM-1、Hcy、MCP-1、ET-1水平:轻度<中度<重度,NO水平:轻度>中度>重度(P<0.05);血清ICAM-1、Hcy、MCP-1水平与ET-1水平成正相关,与NO水平呈负相关(P<0.05)。结论:血清ICAM-1、Hcy、MCP-1水平在RVO患者中均呈异常升高状态,且与ET-1、NO具有一定的相关性,可通过对血清ICAM-1、Hcy、MCP-1水平的检测用以评估血管内皮功能损伤状况,以便于及早实施治疗。

MCP-1及CCR2在初诊弥漫大B细胞淋巴瘤中的表达及临床意义

目的:分析MCP-1及CCR2在初治弥漫大B细胞淋巴瘤(DLBCL)组织中的表达,并评估其与临床病理特征和预后的相关性。方法:回顾性收集2017年1月至2022年5月期间蚌埠医学院第一附属医院血液科确诊及治疗的141例初治DLBCL患者的临床特征、病理学资料,通过免疫组化染色检测MCP-1及CCR2在初治DLBCL患者组织中的表达情况,分析其与患者的临床特征、预后及生存的关系。结果:MCP-1及CCR2的表达与DLBCL患者Ann Arbor分期晚、IPI评分高、乳酸脱氢酶(LDH)升高、Ki-67指数高及疗效差有关,与其他病理学参数(如性别、年龄、β2-微球蛋白、BCL-2、BCL-6、Hans分型、首发部位、有无B症状、骨髓是否受累)均无显著相关性。生存曲线分析显示,MCP-1或CCR2阳性组与阴性组OS及PFS具有统计学差异,且与预后不良有关。单因素Cox回归法分析结果显示,β2-微球蛋白、Ki-67指数、IPI评分、MCP-1、CCR2表达水平对患者的PFS和OS有影响,疗效不佳的患者的PFS和OS明显缩短(P<0.05),性别、年龄、LDH、BCL-2、BCL-6、Hans分型、肿瘤原发部位、有无B症状、骨髓是否受累、Ann Arbor分期对患者的PFS及OS无影响(P>0.05)。多因素分析结果表明,β2-微球蛋白高表达、Ki-67指数高、IPI评分高、MCP-1、CCR2高表达水平及疾病缓解的深度是患者预后不良的独立影响因素(P<0.05)。结论:MCP-1或CCR2在初治DLBCL中表达率高,且与DLBCL患者Ann Arbor分期、IPI评分、LDH及Ki-67指数相关预后差的临床指标有关,是影响PFS和OS的不良预后因素。

黄柏碱调节MCP-1/CCR2信号通路对特应性皮炎大鼠炎症反应的影响

目的:探讨黄柏碱对特应性皮炎(Atopic dermatitis,AD)大鼠炎症反应的影响及其作用机制。方法:构建AD大鼠模型,大鼠分为正常组、模型组、黄柏碱低剂量组、黄柏碱高剂量组、黄柏碱+巨噬细胞趋化蛋白-1(Monocyte chemotactic protein-1,MCP-1)组;给药结束后,各组大鼠做皮损评分,记录搔抓次数,HE染色观察皮肤组织病理变化,甲苯胺蓝染色测定肥大细胞数,ELISA试剂盒测定皮肤组织活性氧(Reactiveoxygenspecies,ROS)和血清免疫球蛋白(Immunoglobulins,IgE)、白介素-17(Interleukin,IL-17)、IL-6的含量,Western blot检测皮肤组织MCP-1、CC类趋化因子受体2(CC chemokinereceptor 2,CCR2)蛋白表达。结果:与正常组相比,模型组大鼠脱毛处皮肤发生溃疡、红斑,表皮和棘层增厚且有大量炎性细胞浸润,搔抓次数、肥大细胞数、ROS、IgE、IL-17、IL-6及MCP-1、CCR2蛋白表达水平增加(P<0.05);与模型组相比,黄柏碱低、高剂量组皮肤组织红斑、溃疡情况、炎性细胞浸润减少,未见脱屑,搔抓次数、肥大细胞数、ROS、IgE、IL-17、IL-6及MCP-1、CCR2蛋白表达水平依次降低(P<0.05);与黄柏碱高剂量组相比,黄柏碱+MCP-1组皮肤红斑、溃疡和炎性细胞浸润加重,搔抓次数、肥大细胞数、ROS、IgE、IL-17、IL-6及MCP-1、CCR2蛋白表达水平增加(P<0.05)。结论:黄柏碱可能通过抑制MCP-1/CCR2信号通路降低AD大鼠炎症反应。

桂枝茯苓汤结合金刚藤胶囊治疗慢性盆腔炎的疗效及对MCP-1、TGF-β1、GM-CSF水平的影响

目的:探讨分析桂枝茯苓汤结合金刚藤胶囊治疗慢性盆腔炎(CPID)的疗效及对单核细胞趋化蛋白1(MCP-1)、转化生长因子-β1(TGF-β1)、粒-巨核细胞集落刺激因子(GM-CSF)水平的影响。方法:回顾选取2022年1月~2024年1月我院妇产科收治的CPID患者共93例,按不同给药方法分为试验组52例和对照组41例。两组均给予奥硝唑联合左氧氟沙星治疗,试验组在此基础上给予桂枝茯苓汤结合金刚藤胶囊进行治疗,比较两组治疗2周后临床疗效、治疗前后中医症候评分、血液流变学[纤维蛋白原(Fib)、血浆粘度、血细胞比容]及血清MCP-1、TGF-β1、GM-CSF的变化。结果:治疗后,试验组临床疗效高于对照组(P<0.05);治疗后,试验组及对照组患者腰腹疼痛、带下量多、疲乏无力等各项中医症候积分相较治疗前均有下降,其中试验组下降更为明显(P<0.05);治疗后,试验组血细胞比容、Fib、血浆粘度相较治疗前明显改善,且改善效果优于对照组(P<0.05);治疗后,试验组血清MCP-1、TGF-β1、GM-CSF明显下降且降幅大于对照组(P<0.05)。结论:桂枝茯苓汤结合金刚藤胶囊治疗CPID,可有效缓解患者临床症状、改善血液流变学并降低血清MCP-1、TGF-β1、GM-CSF水平,临床疗效确切。

Small extracellular vesicles from hypoxia-preconditioned bone marrow mesenchymal stem cells attenuate spinal cord injury via miR-146a-5p-mediated regulation of macrophage polarization

Spinal cord injury is a disabling condition with limited treatment options.Multiple studies have provided evidence suggesting that small extracellular vesicles(SEVs)secreted by bone marrow mesenchymal stem cells(MSCs)help mediate the beneficial effects conferred by MSC transplantation following spinal cord injury.Strikingly,hypoxia-preconditioned bone marrow mesenchymal stem cell-derived SEVs(HSEVs)exhibit increased therapeutic potency.We thus explored the role of HSEVs in macrophage immune regulation after spinal cord injury in rats and their significance in spinal cord repair.SEVs or HSEVs were isolated from bone marrow MSC supernatants by density gradient ultracentrifugation.HSEV administration to rats via tail vein injection after spinal cord injury reduced the lesion area and attenuated spinal cord inflammation.HSEVs regulate macrophage polarization towards the M2 phenotype in vivo and in vitro.Micro RNA sequencing and bioinformatics analyses of SEVs and HSEVs revealed that mi R-146a-5p is a potent mediator of macrophage polarization that targets interleukin-1 receptor-associated kinase 1.Reducing mi R-146a-5p expression in HSEVs partially attenuated macrophage polarization.Our data suggest that HSEVs attenuate spinal cord inflammation and injury in rats by transporting mi R-146a-5p,which alters macrophage polarization.This study provides new insights into the application of HSEVs as a therapeutic tool for spinal cord injury.

Spi1 regulates the microglial/macrophage inflammatory response via the PI3K/AKT/mTOR signaling pathway after intracerebral hemorrhage

Preclinical and clinical studies have shown that microglia and macrophages participate in a multiphasic brain damage repair process following intracerebral hemorrhage.The E26 transformation-specific sequence-related transcription factor Spi1 regulates microglial/macrophage commitment and maturation.However,the effect of Spi1 on intracerebral hemorrhage remains unclear.In this study,we found that Spi1 may regulate recovery from the neuroinflammation and neurofunctional damage caused by intracerebral hemorrhage by modulating the microglial/macrophage transcriptome.We showed that high Spi1expression in microglia/macrophages after intracerebral hemorrhage is associated with the activation of many pathways that promote phagocytosis,glycolysis,and autophagy,as well as debris clearance and sustained remyelination.Notably,microglia with higher levels of Soil expression were chara cterized by activation of pathways associated with a variety of hemorrhage-related cellular processes,such as complement activation,angiogenesis,and coagulation.In conclusion,our results suggest that Spi1 plays a vital role in the microglial/macrophage inflammatory response following intracerebral hemorrhage.This new insight into the regulation of Spi1 and its target genes may advance our understanding of neuroinflammation in intracerebral hemorrhage and provide therapeutic targets for patients with intracerebral hemorrhage.

血清MCP-1和MIP-1β水平与老年脓毒症患者心肌损伤的相关性

目的探讨血清单核细胞趋化因子蛋白1(MCP-1)和巨噬细胞炎性蛋白-1β(MIP-1β)水平与老年脓毒症患者心肌损伤的相关性。方法前瞻纳入2021年3月~2022年3月医院50例出现心肌损伤的老年脓毒症患者,纳入心肌损伤组,同期50例未出现心肌损伤的老年脓毒症患者,纳入非心肌损伤组,测定并比较两组入院时血清MCP-1和MIP-1β水平,分析血清MCP-1和MIP-1β水平与老年脓毒症患者心肌损伤的关系。结果心肌损伤组血清心肌肌钙蛋白T(cTnT)、B型钠尿肽前体(Pro-BNP)、肌酸激酶同工酶(CK-MB)、MCP-1和MIP-1β表达水平高于非心肌损伤组,差异有统计学意义(均P<0.01);经单项Logistic回归分析后建立多元回归模型行多因素分析,结果显示,血清c TnT、Pro-BNP、CK-MB、MCP-1、MIP-1β表达与老年脓毒症患者心肌损伤有关,可能是老年脓毒症患者心肌损伤的预测因素(OR>1,P<0.05);绘制ROC曲线发现,血清MCP-1、MIP-1β表达单独及联合预测老年脓毒症患者心肌损伤的AUC均>0.850,均有一定预测价值。结论血清MCP-1、MIP-1β过表达可能与老年脓毒症患者心肌损伤有关,增加心肌损伤,联合检测老年脓毒症早期血清MCP-1和MIP-1β水平可预测心肌损伤风险。

Mudskipper interleukin-34 modulates the functions of monocytes/macrophages via the colony-stimulating factor-1 receptor 1

Interleukin-34(IL-34)is a novel cytokine that plays an important role in innate immunity and inflammatory processes by binding to the colonystimulating factor-1 receptor(CSF-1R).However,information on the function of IL-34 in fish remains limited.In the present study,we identified an IL-34 homolog from mudskippers(Boleophthalmus pectinirostris).In silico analysis showed that the mudskipper IL-34(BpIL-34)was similar to other known IL-34 variants in sequence and structure and was most closely related to an orange-spotted grouper(Epinephelus coioides)homolog.BpIL-34 transcripts were constitutively expressed in various tissues,with the highest level of expression found in the brain.Edwardsiella tarda infection significantly up-regulated the mRNA expression of BpIL-34 in the mudskipper tissues.The recombinant mature BpIL-34 peptide(rBpIL-34)was purified and used to produce anti-rBpIL-34 IgG.Western blot analysis combined with PNGase F digestion revealed that native BpIL-34 in monocytes/macrophages(MOs/MФs)was N-glycosylated.In vitro,rBpIL-34 treatment enhanced the phagocytotic and bactericidal activity of mudskipper MOs/MФs,as well as the mRNA expression of pro-inflammatory cytokines like tumor necrosis factorα(BpTNF-α)and BpIL-1βin these cells.Furthermore,the knockdown of mudskipper CSF-1R1(BpCSF-1R1),but not mudskipper BpCSF-1R2,significantly inhibited the rBpIL-34-mediated enhanced effect on MO/MФfunction.In conclusion,our results indicate that mudskipper BpIL-34 modulates the functions of MOs/MФs via BpCSF-1R1.

Effects of Leptin on Expression of Acyl-coenzymeA:Cholesterol Acyltransferases-1 in Cultured Human Monocyte-macrophages

Summary: To investigate the effects of leptin on expression of acyl-coenzymeA:cholesterol acyltransferases-1 (ACAT-1) in monocyte-macrophage differentiation, human monocytic cells (THP-1) were cultured in RPMI 1640 and made to differentiate into macrophages under the incubation with phorbol myristate acetate (PMA) for 48 h. The cells were divided into 4 groups according to different intervention factors as follows: MCs cultured in RPMI1640 medium with 10 % FBS for 48 h served as MC group (control group), MCs cultured in medium with serum-free RPMI1640 containing 5 % BSA, 100 nmol/L PMA for 48 h as MP group, MCs cultured in RPMI1640 medium with 10 % FBS, 10 μmol/ml leptin for 48 h as leptin-MC group, and MCs cultured in medium with serum-free RPMI1640 containing 5 % BSA, 100 nmol/L PMA, and 10 μmol/ml leptin for 48 h as leptin-MP group. Immunocytochemistry, reverse transcription polymerase chain reaction (RT-PCR) and Western blot were performed, respectively, to observe the effects of leptin on expression of ACAT-1 in the monocyte-macrophage differentiation. Our results showed that expression of ACAT-1 protein and mRNA in MP-group is two times that in MC-group (P<0.05), and the expression of ACAT-1 protein and mRNA increased by up to 4 folds in leptin-MP group as compared with that of MC group (P<0.01). Thus, our results support the idea that expression of ACAT-1 increases more in cultured human macrophages than in monocytes, and leptin can significantly promote ACAT-1 expression. It was concluded that high expression of ACAT-1 may accelerate the development of human atherogenesis,and leptin might participate in atherogenesis by increasing expression of ACAT-1.

血清CRP/Alb、MMP-2及MCP-1水平与结直肠癌患者腹腔镜根治术后吻合口瘘的关系及其预测价值分析

目的:探究血清C反应蛋白(CRP)/清蛋白(Alb)、基质金属蛋白酶-2(MMP-2)及单核细胞趋化蛋白-1(MCP-1)水平与结直肠癌患者腹腔镜根治术(LRS)后吻合口瘘的关系及其预测价值。方法:纳入2019年2月—2022年10月于我院接受LRS治疗后发生吻合口瘘的41例结直肠癌患者作为观察组。另取同期接受LRS治疗后未发生吻合口瘘的40例结直肠癌患者作为对照组。采用单因素及多因素Logistic回归分析影响结直肠癌患者LRS后吻合口瘘的因素,采用受试者工作特征(ROC)曲线分析各因子预测结直肠癌患者LRS后吻合口瘘的效能。结果:单因素分析发现,血清CRP/Alb、MMP-2及MCP-1水平与结直肠癌患者LRS后吻合口瘘有关(均P<0.05)。经多因素Logistic回归分析发现:血清CRP/Alb、MMP-2及MCP-1水平升高均是结直肠癌患者LRS后吻合口瘘的危险因素(均P<0.05)。经ROC曲线分析发现:血清CRP/Alb、MMP-2及MCP-1水平联合(Log P模型)预测结直肠癌患者LRS后吻合口瘘的效能优于上述三项指标单独预测,曲线下面积(AUC)(0.95CI)为0.863(0.783~0.920)。结论:血清CRP/Alb、MMP-2及MCP-1水平与结直肠癌患者LRS后吻合口瘘密切相关,可作为预测吻合口瘘的辅助指标,且CRP/Alb、MMP-2及MCP-1联合预测价值更高。

血清MIF、MCP-1、suPAR水平与脓毒症严重程度及合并ARDS风险的关系

目的探讨血清巨噬细胞迁移抑制因子(MIF)、单核细胞趋化蛋白-1(MCP-1)、可溶性尿激酶型纤溶酶原激活物受体(suPAR)水平与脓毒症严重程度及合并急性呼吸窘迫综合征(ARDS)风险的关系。方法回顾性分析2022年2月至2023年5月太原钢铁(集团)有限公司总医院收治的86例脓毒症患者的临床资料。依据病情程度不同将患者分为脓毒症组(n=20)、严重脓毒症组(n=48)和脓毒症休克组(n=18)。入院72 h内参考ARDS诊断标准将患者分为ARDS组(n=27)和非ARDS组(n=59)。检测并比较各组脓毒症患者血清MIF、MCP-1、suPAR水平。收集ARDS组与非ARDS组患者年龄、性别、体重指数、合并症、感染类型、既往史、心率、急性生理学和慢性健康状况评价Ⅱ(APACHEⅡ)、脓毒症相关性器官衰竭评价(SOFA)评分、白细胞计数、血乳酸、天冬氨酸转移酶(AST)、丙氨酸转移酶(ALT)、总胆固醇等指标。采用多因素Logistic回归分析对影响脓毒症患者并发ARDS的危险因素进行分析。通过受试者工作特征(ROC)曲线分析血清MIF、MCP-1、suPAR水平预测脓毒症患者并发ARDS的价值。结果脓毒症休克组患者血清MIF、MCP-1、suPAR水平分别为(94.02±10.13)、(506.55±45.15)、(13.89±3.95)ng/mL,均高于脓毒症组[(76.93±7.01)、(148.38±35.74)、(6.07±2.13)ng/mL]和严重脓毒症组[(85.46±8.74)、(327.08±40.62)、(8.42±1.07)ng/mL],而严重脓毒症组患者血清MIF、MCP-1、suPAR水平均高于脓毒症组,差异均有统计学意义(P<0.05)。ARDS组与非ARDS组患者的年龄、性别构成比、体重指数、合并症、感染类型、白细胞计数、心率、吸烟史、饮酒史、血乳酸、AST、ALT、总胆固醇比较,差异均无统计学意义(P>0.05);ARDS组患者APACHEⅡ评分、SOFA评分、有急腹症和胰腺炎占比及血清MIF、MCP-1、suPAR水平均高于非ARDS组,差异均有统计学意义(P<0.05)。经多因素Logistic回归分析结果显示,急腹症、胰腺炎、APACHEⅡ评分、SOFA评分、MIF、MCP-1、suPAR是影响脓毒症患者并发ARDS的独立危险因素(P<0.05)。经ROC曲线分析结果显示,血清MIF、MCP-1、suPAR水平均能预测脓毒症患者ARDS的发生,曲线下面积分别为0.904、0.910、0.917,预测价值较好(P<0.05)。结论血清MIF、MCP-1、suPAR水平与脓毒症患者病情程度、并发ARDS密切相关,且血清MIF、MCP-1、suPAR水平对ARDS的发生有较好的预测价值。

Knockout of C6orf120 in Rats Alleviates Concanavalin A-induced Autoimmune Hepatitis by Regulating Macrophage Polarization

Objective The effect of the functionally unknown gene C6orf120 on autoimmune hepatitis was investigated on C6orf120 knockout rats(C6orf120^(-/-))and THP-1 cells.Method Six–eight-week-old C6orf120^(-/-)and wild-type(WT)SD rats were injected with Con A(16 mg/kg),and euthanized after 24 h.The sera,livers,and spleens were collected.THP-1 cells and the recombinant protein(rC6ORF120)were used to explore the mechanism in vitro.The frequency of M1 and M2 macrophages was analyzed using flow cytometry.Western blotting and PCR were used to detect macrophage polarization-associated factors.Results C6orf120 knockout attenuated Con A-induced autoimmune hepatitis.Flow cytometry indicated that the proportion of CD68^(+)CD86^(+)M1 macrophages from the liver and spleen in the C6orf120^(-/-)rats decreased.C6orf120 knockout induced downregulation of CD86 protein and the mRNA levels of related inflammatory factors TNF-α,IL-1β,and IL-6 in the liver.C6orf120 knockout did not affect the polarization of THP-1 cells.However,rC6ORF120 promoted the THP-1 cells toward CD68^(+)CD80^(+)M1 macrophages and inhibited the CD68^(+)CD206^(+)M2 phenotype.Conclusion C6orf120 knockout alleviates Con A-induced autoimmune hepatitis by inhibiting macrophage polarization toward M1 macrophages and reducing the expression of related inflammatory factors in C6orf120^(-/-)rats.

Egr-1 Mediates Si0_2-driven Transcription of Membrane Type Ⅰ Matrix Metalloproteinase in Macrophages

The up-regulation mechanism of membrane type Ⅰ matrix metalloproteinase （MTI-MMP） in macrophages stimulated by silica in vitro and the contribution of early growth response 1 （Egr-1） transcription factor in the gene expression pathway were investigated. Macrophages stimulated by silica were treated with Egr-1 antibody or Egr-1 decoy oligodeoxynucleotides （ODN）. The levels of MT1-MMP proteins were determined by Western blot and the expression of MT1-MMP mRNAs was detected by RT-PCR. The results showed as compared with control macrophages, silica-stimulated group showed up-regulated gene expression of MT1-MMP via Egr-1 （P〈0.01）. Compared with silica-stimulated macrophages untreated with antibody, the cells treated with 5 μg/mL Egr-1 antibody were associated with reduced expression of MTI-MMP protein （P〈0.01） and mRNA （P〈0.01）. Compared with silica-stimulated untransfected group, the Egr-1 ＂decoy＂ ODN group was associated with reduction in the expression of MT1-MMP protein and mRNA （P〈0.01）. It was concluded gene expression of MT1-MMP which may play a critical role in silicosis was up-regulated by silica in macrophages. Egr-1 participated in the expression of MT1-MMP and positively regulated the expression. Both Egr-1 antibody and Egr-1 decoy ODN suppressed the expression of MTI-MMP through the Egr-1 pathway and may become a potential therapeutic tool in the management of silicosis in the future.

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.

ATAT1 deficiency enhances microglia/macrophage-mediated erythrophagocytosis and hematoma absorption following intracerebral hemorrhage

MIcroglia/macrophage-mediated erythrophagocytosis plays a crucial role in hematoma clearance after intracerebral hemorrhage.Dynamic cytoskeletal changes accompany phagocytosis.However,whether and how these changes are associated with microglia/macrophage-mediated erythrophagocytosis remain unclear.In this study,we investigated the function of acetylatedα-tubulin,a stabilized microtubule form,in microglia/macrophage erythrophagocytosis after intracerebral hemorrhage both in vitro and in vivo.We first assessed the function of acetylatedα-tubulin in erythrophagocytosis using primary DiO GFP-labeled red blood cells co-cultured with the BV2 microglia or RAW264.7 macrophage cell lines.Acetylatedα-tubulin expression was significantly decreased in BV2 and RAW264.7 cells during erythrophagocytosis.Moreover,silencingα-tubulin acetyltransferase 1(ATAT1),a newly discoveredα-tubulin acetyltransferase,decreased Ac-α-tub levels and enhanced the erythrophagocytosis by BV2 and RAW264.7 cells.Consistent with these findings,in ATAT1-/-mice,we observed increased ionized calcium binding adapter molecule 1(Iba1)and Perls-positive microglia/macrophage phagocytes of red blood cells in peri-hematoma and reduced hematoma volume in mice with intracerebral hemorrhage.Additionally,knocking out ATAT1 alleviated neuronal apoptosis and pro-inflammatory cytokines and increased anti-inflammatory cytokines around the hematoma,ultimately improving neurological recovery of mice after intracerebral hemorrhage.These findings suggest that ATAT1 deficiency accelerates erythrophagocytosis by microglia/macrophages and hematoma absorption after intracerebral hemorrhage.These results provide novel insights into the mechanisms of hematoma clearance and suggest ATAT1 as a potential target for the treatment of intracerebral hemorrhage.

The expression of chemokine MCP-1 in colorectal carcinoma and its relationship to the infiltration of macrophage

Objective: To study the expression of MCP-1 in colorectal carcinoma and its relationship to the infiltration of the macrophage and to the biological behaviour of infiltration and metastasis of colorectal carcinoma. Methods: The expression of the MCP-1 mRNA was assessed in colorectal carcinoma collected freshly from surgical specimen by RT-PCR and the expres- sion of the MCP-1 protein was assessed in colorectal carcinoma collected from surgical specimen by immunohistochemistry. The tumor infiltrating cell and macrophage were also investigated by immunohistochemistry. Results: All the 12 specimens of colorectal carcinoma detected by RT-PCR expressed the MCP-1 mRNA; MCP-1 protein was detected in 90℅ (36/40) cases of the tumor; The expression of the MCP-1 protein in colorectal carcinoma correlated negatively with its state of metastasis and the Dukes’ stage. But a postive correlation was found between the expression of MCP-1 and the infiltrated macrophage. The stron- ger expression of MCP-1, the more number of the infiltrated macrophage. Conclusion: The expression of chemokine MCP-1 in colorectal carcinoma may influence its biological behaviour of infiltration and metastasis, and can attract the immuno-cell to the local of the tumor, such as Macrophage.