采高1 m的薄煤层大功率采煤机研制

在分析了国内外现有1 m采高薄煤层采煤机的基础上,研制了一种适用于采高1 m的薄煤层大功率采煤机,详细介绍了该采煤机的主要技术参数、关键技术和使用情况,该采煤机成功解决了1 m薄煤层工作面的高效开采问题。

Scavenger receptor A-mediated nanoparticles target M1 macrophages for acute liver injury

Acute liver injury(ALI)has an elevated fatality rate due to untimely and ineffective treatment.Although,schisandrin B(SchB)has been extensively used to treat diverse liver diseases,its therapeutic efficacy on ALI was limited due to its high hydrophobicity.Palmitic acid-modified serum albumin(PSA)is not only an effective carrier for hydrophobic drugs,but also has a superb targeting effect via scavenger receptor-A(SR-A)on the M1 macrophages,which are potential therapeutic targets for ALI.Compared with the common macrophage-targeted delivery systems,PSA enables site-specific drug delivery to reduce off-target toxicity.Herein,we prepared SchB-PSA nanoparticles and further assessed their therapeutic effect on ALI.In vitro,compared with human serum albumin encapsulated SchB nanoparticles(SchB-HSA NPs),the SchB-PSA NPs exhibited more potent cytotoxicity on lipopolysaccharide(LPS)stimulated Raw264.7(LAR)cells,and LAR cells took up PSA NPs 8.79 times more than HSA NPs.As expected,the PSA NPs also accumulated more in the liver.Moreover,SchB-PSA NPs dramatically reduced the activation of NF-κB signaling,and significantly relieved inflammatory response and hepatic necrosis.Notably,the high dose of SchB-PSA NPs improved the survival rate in 72 h of ALI mice to 75%.Hence,SchB-PSA NPs are promising to treat ALI.

血清TGF-β1、FOXM1 mRNA表达水平与支气管哮喘患儿气道重塑的影响研究

目的探讨血清转化生长因子-β1(TGF-β1)、叉头框蛋白M1(FOXM1)mRNA表达水平与支气管哮喘(BA)患儿气道重塑的影响。方法选取2020年8月至2021年9月我院收治的110例BA患儿作为本次研究对象,依据《儿童支气管哮喘诊断与防治指南(2016年版)》将110例BA患儿分为急性发作组(n=56)和临床缓解组(n=54)。对两组的血清TGF-β1、FOXM1 mRNA、气道重塑相关指标(T/D、WA)、肺功能相关指标(FEV1、FEV1/FVC)水平进行检测并比较。采用Pearson分析急性发作期BA患儿血清TGF-β1、FOXM1 mRNA水平和肺功能及气道重塑指标的相关性。通过多因素Logistic回归分析方法分析影响BA患儿急性发作的因素,建立风险评估模型,经受试者工作特征曲线(ROC)评估模型诊断效能。结果与临床缓解组相比较,急性发作组血清TGF-β1、FOXM1 mRNA水平和T/D、WA水平较高,FEV1、FEV1/FVC水平较低(P<0.05);Pearson分析结果表明,急性发作期BA患儿血清TGF-β1、FOXM1 mRNA水平和FEV1、FEV1/FVC水平呈负相关(r=-0.527、r=-0.496,r=-0.492,r=-0.486,P<0.05),与T/D、WA呈正相关(r=0.434,r=0.511,r=0.515,r=0.524,P<0.05);多因素Logistic回归分析结果显示,血清TGF-β1(P=0.029,OR=11.382)、FOXM1 mRNA(P=0.007,OR=3.200)、T/D(P=0.001,OR=3.019)、WA(P=0.004,OR=2.489)水平是BA患儿急性发作的独立影响因素;ROC曲线分析结果表明,上述四种指标联合检测的AUC值最高,为0.997,灵敏度、特异度分别为96.42%、92.85%。结论BA患儿的血清TGF-β1、FOXM1 mRNA表达水平和气道重塑有紧密关联,血清TGF-β1、FOXM1 mRNA水平的提升可在一定程度上引发气道重塑。同时血清TGF-β1、FOXM1 mRNA水平在评估BA患儿病情严重程度方面具有一定的临床应用价值。

重型绞吸挖泥船1 m直径排泥管线输送微风化岩特性

以国外某疏浚工程为例,对自航式重型绞吸挖泥船“天鲲号”采用1 m管径的排泥管线输送坚硬微风化岩的施工数据进行分析,计算所给工况下的泥泵扬程和泥泵效率,得出密度、流速与摩阻系数的关系,给出土质换算系数、实验系数的推荐值。结果表明,该技术充分发挥重型绞吸船可直接开挖并吹填微风化岩的特点,在节约成本、保护环境的基础上提高施工效率,确保工程按期完工。

RANKL-induced M1 macrophages are involved in bone formation

The activation of M1 macrophages can be achieved by stimulating them with lipopolysaccharide （LPS） and interferon-γ （IFN-γ）. However, M1 can be found under physiological conditions without any pathological stimuli. This study aimed to understand the involvement of RANKL-induced M1 macrophages in bone formation compared with pathologically induced macrophages. Fischer rats were used to investigate macrophage distribution in normal and injured femoral condyles in vivo. Bone marrow-derived macrophages （BMDMs） were activated with LPS＋IFN-γ and RANKL to achieve M1 activation in vitro. Gene expression related to inflammation, osteoclastogenesis, angiogenesis, and migration was determined by reverse transcription-quantitative polymerase chain reaction （RT-qPCR） and fluorescence-activated cell sorting （FACS）. Tissue macrophages showed distinct expression patterns at different bone regions. RANKL was found in close proximity to inducible nitric oxide synthase-positive （iNOS＋） cells in vivo, suggesting an association between RANKL expression and iNOS＋ cells, especially in trabecular bone. RANKL-induced macrophages showed a different cytokine secretion profile compared with pathologically induced macrophages. Both osteoclasts and M1 macrophages peaked on day 7 during bone healing. RANKL could trigger Ml-like macrophages with properties that were different from those of LPS＋IFN-γ-induced macrophages. These RANKL-activated M1 macrophages were actively involved in bone formation.

肾疏宁对肾小管间质损害大鼠FN、ColⅢ、PAI-1 mRNA的作用

目的：观察肾疏宁对肾小管间质损害大鼠FN、colm、PAl—lmRNA表达的影响。方法：在系膜增生性肾炎（MsPGN）模型基础上。延长造模时间至12～16周，使其自然发展成肾小管间质损害模型，观察肾疏宁对肾小管间质FN、colm、PAl—lmRNA表达的影响，并设苯那普利为阳性对照组。结果：第12～16周末，造模各组肾小管间质FN、ColⅢ、PAI-1mRNA表达量均明显升高（P〈0．05或P〈0．01），肾疏宁组、苯那普利组均显著低于模型组（P〈0．05或P〈0．01），第12周末，肾疏宁组与苯那普利组比较无统计学差异（P〉0．05），而第16周末，肾疏宁组明显低于苯那普利组（P〈0．01）。结论：肾疏宁能抑制细胞外基质的合成，促进其降解，从而保护肾小管间质损害。

HL-1 M装置低杂波注入的边缘等离子体特性

利用多组马赫 朗缪尔探针测量HL 1M装置刮离层和边缘的雷诺胁强、等离子体极向旋转、径向和极向电场的变化。在低杂波注入实验中 ,改变低杂波驱动功率 ,从而改变边缘电场、等离子体旋转速度和边缘静电雷诺胁强。结果指出 ,在托卡马克等离子体边缘 ,雷诺胁强的径向变化可以产生剪切极向流。

人造板甲醛释放量1 m^(3)气候箱法的方法检出限评估

依据GB/T 27417—2017《合格评定化学分析方法确认和验证指南》中空白标准偏差法,对GB/T 17657—2013《人造板及饰面人造板理化性能试验方法》中人造板甲醛释放量1 m^(3)气候箱法的方法检出限进行评估,得到其检出限为0.006 mg/m^(3),为人造板甲醛释放量检验检测提供参考。

血管紧张素Ⅱ对RIN-m细胞PDX-1 mRNA及蛋白表达的影响

目的探讨血管紧张素Ⅱ(ATⅡ)对胰十二指肠同源盒1(PDX-1)表达的影响及其与胰岛素(Ins)分泌的关系。方法测定RIN-m细胞在基础、ATⅡ及氯沙坦作用下Ins分泌量、细胞内Ins含量及细胞内PDX-1 mRNA和蛋白的表达水平。结果在100nmol/LATⅡ作用下,葡萄糖刺激后Ins分泌量、细胞内Ins含量及PDX-1表达水平均明显降低(P均<0.05)。上述作用可被ATⅡ受体阻滞剂氯沙坦部分逆转。结论抑制PDX-1表达水平可能是ATⅡ影响胰岛β细胞Ins合成及分泌的机制之一。

miR-370-3p和FOXM1 mRNA对人成骨肉瘤细胞增殖、迁移、侵袭的影响观察及其靶向关系验证

目的观察骨肉瘤组织中miR-370-3p、FOXM1 mRNA的表达,观察miR-370-3p和FOXM1 mRNA对人成骨肉瘤细胞系MG63增殖、迁移及侵袭的影响,并验证其靶向关系机制。方法①观察骨肉瘤及癌旁组织miR-370-3p及及其下游靶基因叉头框蛋白M1(FOXM1)mRNA表达:37例骨肉瘤患者,均行肿瘤切除术,术中保存骨肉瘤及癌旁组织,采用实时定量PCR法检测骨肉瘤及癌旁组织miR-370-3p、FOXM1 mRNA,分析骨肉瘤组织FOXM1 mRNA表达与miR-370-3p表达的相关性。采用Kaplan-Meier曲线、Log-Rank检验分析miR-370-3p表达与骨肉瘤患者临床病理参数及预后关系。②观察miR-370-3p过表达及FOXM1抑制表达的人成骨肉瘤细胞系MG63增殖、迁移及侵袭的影响:取MG63细胞分为1~4组,分别转染miR-370-3p mimic(促进miR-370-3p表达)、mimic NC(空载体质粒)、空白对照组及FOXM1 siRNA干扰质粒(FOXM1基因敲除质粒)。分别于转染0、24、48、72、96 h采用CCK-8法观察各组细胞增殖情况,采用划痕实验观察各组细胞迁移情况,采用Transwell小室观察各组细胞侵袭能力。③预测MG63细miR-370-3p与FOXM1靶向关系构建pmirGLO-FOXM1-野生型/突变型质粒,将MG63细胞分为A、B、C、D组,分别用1μL pmirGLO-FOXM1-WT+200 nmol miR-370-3p mimic、1μL pmirGLO-FOXM1-WT+mimic NC、1μL pmirGLO-FOXM1-MUT+200 nmol miR-370-3p mimic、1μL pmirGLO-FOXM1-MUT+200 nmol mimic NC转染。转染24 h时采用双荧光素酶报告检测系统观察各组细胞荧光活性。结果①与癌旁组织比较,骨肉瘤组织miR-370-3p相对表达量低、FOXM1 mRNA相对表达量高(t=4.66,3.41;P均<0.05)。随miR-370-3p表达量升高,骨肉瘤组织FOXM1 mRNA表达量呈下降趋势(R2=0.6481,P=0.1284)。miR-370-3p表达与骨肉瘤患者临床分期、远端转移情况有关(χ2=4.430、6.027;P均<0.05)。miR-370-3p低表达的骨肉瘤患者预后比miR-370-3p高表达患者差(P<0.05)。②2、3组相比,转染48、72、96 h时1、4组细胞OD450值均降低(P均<0.05)。与2、3组相比,转染24 h时1、4组划痕愈合率低、穿膜细胞数少(P均<0.05)。③与B组比较,A组细胞荧光活性降低(P<0.05);与D组比较,C组细胞中荧光活性变化不明显(P>0.05)。结论骨肉瘤组织中miR-370-3p表达降低、FOXM1 mRNA表达升高。促进miR-370-3p表达及FOXM1抑制表达的MG63细胞增殖、侵袭及迁移能力均降低。骨肉瘤细胞中miR-370-3p可能通过靶向调控FOXM1表达来抑制MG63的增殖、迁移及侵袭。

Tramadol in Japanese Population: the Relative Contribution of M1 Metabolite as Assessed by <i>CYP</i>2<i>D</i>6</i>*10 Genotype

Several preclinical and clinical studies suggested that tramadol has a multi-mechanistic analgesic action. Upon in vitro evaluation, tramadol parent drug was determined to have only very weak affinity for opioid receptors. Metabolism via CYP2D6, though, yields the O-desmethyl metabolite (M1), which has much greater opioid receptor affinity. In tests in animals and human volunteers, tramadol’s analgesic effect is only partially blocked by the opioid antagonist naloxone. Yet the contribution of parent drug to analgesia is still debated. Observance of good analgesic response to tramadol in Japanese and other Asian populations that express the CYP2D6*10 genotype suggests that parent drug accounts for the majority of tramadol’s analgesic effect in most clinical settings. Understanding of tramadol’s multi-mechanistic action continues to form the basis for understanding its clinical attributes.

铂类治疗卵巢癌患者外周血XRCC1、ERCC1、RRM1 mRNA和蛋白的检测及其意义研究

目的检测上皮源性卵巢癌患者外周血X射线交错互补修复基因1(XRCC1)、核苷酸切除修复交叉互补基因1(ERCC1)和核糖核苷还原酶调节因子M1(RRM1)mRNA和蛋白的表达情况,并进行铂类耐药的相关性评价。方法收集66例卵巢上皮性恶性肿瘤患者,术后接受6～8个疗程的铂类药物化疗,根据美国国立综合癌症网络(NCCN)指南分为铂类敏感组(19例)、铂类部分敏感组(25例)及铂类耐药组(22例),采用ELISA方法检测血清中XRCC1、ERCC1和RRM1蛋白的表达,real time PCR法检测患者外周血中XRCC1、ERCC1和RRM1 mRNA的表达。结果三组患者XRCC1、ERCC1和RRM1蛋白在血清中的表达均呈上升趋势(P<0.05)。铂类部分敏感组和铂类耐药组XRCC1、ERCC1、RRM1蛋白的表达高于铂类敏感组(P<0.05);铂类耐药组XRCC1、ERCC1、RRM1蛋白的表达水平高于铂类部分敏感组(P<0.05)。real time PCR结果表明ERCC1和XRCC1 mRNA表达水平在三组中呈逐渐上升的趋势(P<0.05),而RRM1 mRNA表达水平则呈逐渐下降的趋势(P<0.05),与铂类敏感组比较,铂类部分敏感组ERCC1和RRM1 mRNA表达水平差异无统计学意义(P>0.05),XRCC1 mRNA表达水平增高(P<0.05);铂类耐药组XRCC1和ERCC1 mRNA呈高水平表达(P<0.05),RRM1 mRNA呈低水平表达(P<0.05)。与铂类部分敏感组比较,铂类耐药组XRCC1和ERCC1mRNA表达水平增高(P<0.05),RRM1 mRNA表达水平降低(P<0.05)。相关性分析表明,铂类耐药组RRM1mRNA和蛋白表达无相关性(P>0.05),XRCC1、ERCC1 mRNA和蛋白表达呈正相关(P<0.05)。结论外周血XRCC1、ERCC1、RRM1基因表达可能影响卵巢癌顺铂化疗治疗的敏感性。

关于二重递归数列{A_m^n}_(n=1 m=1)~∞的通项公式的两个定理

关于满足条件am+k=λ1an+k-1+λ2a（n+k-2）+…λkan的一元线性递归数列{an}的通项公式,已经有了很好的结论。本文对二重数列及满足简单条件Amn=λ1Am-1n+λ2Am-1n-1的二重线性递归数列的通项公式得到两个有用的定理。

超声造影联合血清Ficolin-3,FOXM1对2型糖尿病下肢动脉病变的诊断价值分析

目的超声造影联合血清纤维胶凝蛋白-3(Ficolin-3)、叉头框蛋白M1(FOXM1)对2型糖尿病(T2DM)下肢动脉病变的诊断价值分析。方法选取2022年2月至2023年2月我院收治的T2DM患者114例,以下肢动脉血管造影检查为金标准,将患者分为下肢动脉病变组23例(病变组)和无下肢动脉病变组91例(T2DM组),另选取同期于本院进行体检的健康志愿者91例为对照组。对患者及健康志愿者进行血清Ficolin-3、FOXM1及超声造影检查;ROC曲线分析血清Ficolin-3、FOXM1对T2DM下肢动脉病变的诊断价值;采用四格表法分析血清Ficolin-3、FOXM1、超声造影及3项联合对T2DM下肢动脉病变的诊断价值。结果病变组、T2DM组血清Ficolin-3水平显著高于对照组,且病变组血清Ficolin-3水平显著高于T2DM组(均P<0.05);病变组、T2DM组血清FOXM1水平显著低于对照组,且病变组血清FOXM1水平显著低于T2DM组(均P<0.05);血清Ficolin-3诊断T2DM下肢动脉病变的曲线下面积为0.868,敏感度为86.96%,特异度为75.82%,最佳截断值为35.12μg/ml;血清FOXM1诊断T2DM下肢动脉病变的曲线下面积为0.854,敏感度为82.61%,特异度为78.02%,最佳截断值为0.57;血清Ficolin-3、FOXM1检查结果与金标准均具有中度一致性(Kappa=0.480、0.481,均P<0.001);超声造影检查结果显示,T2DM下肢动脉病变的阳性检出率为73.91%,与金标准具有较高一致性(Kappa=0.631,P<0.001);3项联合检测的敏感度、漏诊率均显著优于超声造影单独诊断,准确度显著优于Ficolin-3、FOXM1单独诊断,差异均有统计学意义(均P<0.05)。结论血清Ficolin-3、FOXM1联合超声造影检查在T2DM下肢动脉病变诊断中的应用价值较高,进一步提升了诊断的敏感度、准确度,减少了误诊率。

中药通心络胶囊对糖尿病足大鼠nephrin、podocin 水平、巨噬细胞M1表型及VEGF蛋白的作用

目的研究中药通心络胶囊对糖尿病足大鼠nephrin、podocin水平、巨噬细胞M1表型及血管内皮生长因子(VEGF)蛋白的作用。方法SPF级健康SD大鼠50只,随机抽取10只作为健康组进行对照,剩余40只进行糖尿病足模型建立,建模成功后40只大鼠按随机数字表法分为模型组,通心络低、中、高剂量组,每组10只,健康组、模型组给予2 ml生理盐水灌胃;通心络低、中、高剂量组分别给予通心络胶囊0.50、0.75、1.00 g/kg灌胃。苏木素-伊红(HE)染色观察大鼠肾组织病理形态,HE及Masson染色观察大鼠足部病理形态,RT-聚合酶链反应(PCR)检测Nephrin、podocin表达,多重免疫荧光检测伤口组织中M1型和M2型巨噬细胞数量,Western印迹检测细胞中VEGF、缺氧诱导因子(HIF)-1α蛋白表达水平,应用ImageJ 1.46医学图像分析糖尿病足大鼠溃疡面积。结果模型组肾小球萎缩,基底膜增厚,有炎性细胞浸润,足部炎症细胞较多,新生胶原纤维组织较薄,且排列疏松、不规律,管腔较少;与模型组相比,通心络低、中、高剂量组有所改善。与健康组相比,模型组nephrin、podocin、VEGF、HIF-1α水平显著降低;与模型组相比,通心络各剂量组nephrin、podocin、VEGF、HIF-1α水平显著升高,且以高剂量组效果最为显著(P<0.05)。与模型组相比,通心络低、中、高剂量组M1型巨噬细胞显著减少、M2型巨噬细胞数目显著增多(P<0.05)。结论通心络胶囊可促进VEGF/HIF-1α表达,使巨噬细胞向M1极化,从而促进创面愈合,提高nephrin/podocin表达水平,减轻由糖尿病足导致的肾脏负担。

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.

小檗碱联合姜黄素调控M1巨噬细胞极化对动脉粥样硬化的作用机制

目的探究小檗碱联合姜黄素通过介导巨噬细胞向M1极化对动脉粥样硬化(AS)的作用及机制。方法常规培养小鼠单核巨噬细胞(RAW264.7),通过脂多糖(LPS,100 ng/mL)和γ干扰素(IFN-γ)(20 ng/mL)诱导巨噬细胞RAW264.7获得M1型巨噬细胞,建立细胞模型。将细胞分为对照组、模型组、小檗碱组、姜黄素组、小檗碱+姜黄素联合治疗组。通过CCK-8方法检测小檗碱和姜黄素的处理浓度。ELISA检测各组巨噬细胞上清液M1型巨噬细胞标记物iNOS、TNF-α、CXCL9和p-STAT6/STAT6的表达水平;RT-PCR方法检测iNOS、TNF-α和CXCL9 mRNA水平;Western blot检测各组iNOS、STAT6和p-STAT6蛋白水平。此外,通过siRNA技术下调STAT6水平后,通过Western blot检测p-STAT6蛋白水平的表达;ELISA检测iNOS、TNF-α、CXCL9和p-STAT6表达水平。结果LPS和IFN-γ联合诱导M1巨噬细胞极化中,相较于其他药物浓度组比,小檗碱(25μmol/L)、姜黄素(20μmol/L)为最佳药物浓度,两者单用和联用均不能显著抑制RAW264.7细胞活力(P<0.05)。与正常组比较,模型组iNOS、TNF-α和CXCL9 mRNA和蛋白水平均升高,p-STAT6/STAT6水平降低,差异有统计学意义(P<0.05);与模型组相比,小檗碱组、姜黄素组、小檗碱+姜黄素联合治疗组中iNOS、TNF-α和CXCL9 mRNA和蛋白水平均降低,p-STAT6/STAT6水平升高,且小檗碱+姜黄素联合治疗组中变化的更加明显,差异有统计学意义(P<0.05)。在小檗碱+姜黄素联合治疗组的M1型巨噬细胞中转染STAT6 siRNA后可下调p-STAT6水平,上调iNOS、TNF-α和CXCL9表达,差异有统计学意义(P<0.05)。结论小檗碱和姜黄素对M1型巨噬细胞的活性均有抑制作用,能够减轻炎症反应。此外,小檗碱与姜黄素联合作用较单药使用更有优势,可能是通过活化STAT6发挥其主要作用机制。

Picroside Ⅱ promotes HSC apoptosis and inhibits the cholestatic liver fibrosis in Mdr2^(−/−)mice by polarizing M1 macrophages and balancing immune responses

Liver fibrosis is characterized by chronic inflammatory responses and progressive fibrous scar formation.Macrophages play a central role in the pathogenesis of hepatic fibrosis by reconstructing the immune microenvironment.Picroside Ⅱ(PIC Ⅱ),extracted from Picrorhizae Rhizoma,has demonstrated therapeutic potential for various liver damage.However,the mechanisms by which macrophage polarization initiates immune cascades and contributes to the development of liver fibrosis,and whether this process can be influenced by PIC Ⅱ,remain unclear.In the current study,RNA sequencing and multiple molecular approaches were utilized to explore the underlying mechanisms of PIC Ⅱ against liver fibrosis in multidrug-resistance protein 2 knockout(Mdr2^(−/−))mice.Our findings indicate that PIC Ⅱ activates M1-polarized macrophages to recruit natural killer cells(NK cells),potentially via the CXCL16-CXCR6 axis.Additionally,PIC Ⅱ promotes the apoptosis of activated hepatic stellate cells(aHSCs)and enhances the cytotoxic effects of NK cells,while also reducing the formation of neutrophil extracellular traps(NETs).Notably,the anti-hepatic fibrosis effects associated with PIC Ⅱ were largely reversed by macrophage depletion in Mdr2^(−/−)mice.Collectively,our research suggests that PIC Ⅱ is a potential candidate for halting the progression of liver fibrosis.

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.