抗IL-13单抗抑制上呼吸道杯状细胞增生缓解急性声门下喉炎的疗效及分子机制研究

目的探讨抗白细胞介素(IL)-13单抗通过缓解杯状细胞化生及增生在急性声门下喉炎治疗中的作用及其分子机制。方法采集海南医学院第一附属医院收治的33例临床急性声门下喉炎患儿的外周血标本,根据Westley哮喉评分将患儿分为轻度组(Mild group)和中-重度组(Moderate-Severe group)。体外在气/液界面(ALI)培养正常人支气管上皮细胞(NHBE细胞),细胞实验分组:Group-1(对照组,NHBE细胞维持培养)、Group-2(纤毛细胞诱导组)、Group-3(IL-13处理组)、Group-4(IL-13+抗IL-13单抗处理组)。采用酶联免疫吸附试验(ELISA)测定外周血血清或细胞培养上清液炎症因子IL-10、干扰素γ(IFN-γ)和IL-13水平。采用免疫印迹(Western blot)法测定杯状细胞分化标志物麦芽凝集素(WGA)和纤毛细胞分化标志物乙酰化-α-微管蛋白(AAT)的表达水平,以及磷酸化(p-)胞外信号调节蛋白激酶1/2(ERK1/2)和ERK1/2的表达水平,采用光学显微镜测量细胞直径。在体动物实验中,将30只雌性C57BL/6J小鼠随机分为Control组、Model组[使用卵清蛋白(OVA)+脂多糖(LPS)诱导哮喘小鼠模型]和Model+anti-IL-13 antibody组(鼻滴法给予Model组小鼠抗IL-13单抗治疗),每组10只。结果与Mild group相比,Moderate-Severe group外周血血清IL-10、IFN-γ和IL-13水平均升高(P<0.05)。与Group-1细胞相比,Group-2 AAT表达水平上调(P<0.05);Group-3 WGA表达水平上调(P<0.05),IL-10、IFN-γ和IL-13水平升高(P<0.05),杯状细胞直径增大(P<0.05),p-ERK1/2水平上调(P<0.05);与Group-3相比,Group-4 WGA表达水平下调(P<0.05),IL-10、IFN-γ和IL-13水平降低(P<0.05),杯状细胞直径减小(P<0.05),p-ERK1/2水平下调(P<0.05)。4组细胞ERK1/2表达水平差异无统计学意义(P>0.05)。在体动物实验结果显示,与Control组小鼠相比,Model组小鼠支气管炎症评分升高(P<0.05);与Model组相比,Model+anti-IL-13 antibody组小鼠支气管炎症评分降低(P<0.05)。结论抗IL-13单抗可抑制气道杯状细胞化生和增生,或许可用于缓解急性声门下喉炎。

香加皮乙酸乙酯提取物诱导人食管癌TE-13细胞凋亡的作用机制

目的:研究香加皮乙酸乙酯提取物(ethyl acetate extract fromCortex periplocae,CPEAE)诱导人食管癌细胞TE-13凋亡的作用机制。方法:采用MTT法分析CPEAE对TE-13细胞增殖的抑制作用;Giemsa染色法和透射电子显微镜下观察CPEAE处理后细胞凋亡形态的变化;FCM法检测CPEAE对细胞周期和凋亡率的影响;Western印迹法检测用药前后TE-13细胞中CDK4蛋白表达的变化。结果:CPEAE抑制TE-13细胞的增殖(P<0.05),并呈浓度及时间依赖性,作用48 h时的IC50值为(2.443±0.005)μg/mL;透射电子显微镜下观察发现,TE-13细胞发生了特征性的凋亡形态学改变;FCM检测可见典型的凋亡峰;CPEAE作用TE-13细胞后,CDK4基因表达水平降低。结论:CPEAE可诱导TE-13细胞发生凋亡,可能是通过下调CDK4基因表达水平而实现的。

反义寡核苷酸沉默乙酰肝素酶对食管鳞癌细胞株TE-13侵袭能力的影响

背景与目的:乙酰肝素酶(heparanase,Hpa)为降解硫酸乙酰肝素多糖的内糖苷酶,在多种恶性肿瘤的侵袭转移中发挥重要作用。本研究旨在探讨Hpa在食管鳞癌细胞株TE-13中的表达和转染Hpa反义寡核苷酸(antisenseoligodeoxynucleotide,ASODN)对TE-13细胞的影响。方法:脂质体法转染人工合成的HpaASODN片段,应用RT-PCR、Westernblot和免疫细胞化学方法检测转染前后Hpa基因和蛋白表达的变化,Matrigel侵袭实验观察转染ASODN后TE-13细胞侵袭行为的改变。结果:在TE-13细胞中,RT-PCR扩增得到大小为585bp的Hpa基因条带,Westernblot检测到50ku大小的Hpa蛋白,免疫细胞化学染色表明Hpa主要定位于胞浆和胞膜。转染不同浓度HpaASODN后,RT-PCR、Westernblot和细胞免疫染色均证实TE-13细胞Hpa基因和蛋白表达下调,且随HpaASODN的浓度增高,基因和蛋白表达量逐渐降低(P<0.05),不同浓度HpaASODN组间有显著性差异(P<0.05)。Matrigel侵袭实验中,转染不同浓度HpaASODN后,侵袭至下室面的TE-13细胞数均下降(P<0.05)。随HpaASODN浓度的增高,侵袭至下室面的TE-13细胞个数逐渐减少(P<0.05),不同浓度HpaASODN组间有显著性差异(P<0.05)。结论:TE-13细胞存在Hpa基因的表达。HpaASODN能显著降低Hpa基因表达量,并且使TE-13细胞侵袭力明显下降。

对羟基桂皮醛诱导食管癌TE-13细胞分化及其作用机制

目的:探讨木鳖子单体化合物对羟基桂皮醛(p-hydroxylcinnamaldehyde,CMSP)对食管癌细胞株TE-13的分化作用及其机制。方法:用流式细胞术检测质量浓度为10、20、40Dμg/ml的CMSP处理TE-13细胞对该细胞凋亡和细胞周期分布的影响,用吉姆萨染色、电镜观察TE-13细胞形态学改变,Real-time PCR和ELISA方法检测TE-13细胞中肿瘤相关抗原CEA和SCC的表达,用克隆集落形成实验、Transwell迁移实验检测不同质量浓度CMSP对TE-13细胞的增殖、迁移能力的影响,Western blotting检测CMSP(20μg/ml)对TE-13细胞中MAPK通路中各蛋白水平的影响。结果:CMSP可抑制食管癌Kyse30、TE-13、Eca109和Kyse180细胞的增殖[(1.6±0.2)×10~4 vs(3.8±0.3)×10~4、(1.7±0.3)×10~4 vs(4.5±0.4)×10~4、(2.5±0.1)×10~4 vs(4.0±0.4)×10~4、(1.5±0.1)×10~4vs(2.5±0.3)×10~4个细胞,均P<0.01],而对人食管上皮细胞无明显作用(P>0.05)。CMSP处理TE-13细胞后:(1)随CMSP质量浓度(10、20、40μg/ml)和处理时间的增加(24、48、72 h),G_0/G_1期细胞数量均增加、S期细胞数量减少(P<0.01或P<0.05),但细胞凋亡率无明显变化(P>0.05);(2)细胞出现典型分枝状突起,且随CMSP质量浓度增加更显著(P<0.05);(3)CEA和SCC水平显著降低(P<0.01);(4)抑制TE-13细胞的增殖和迁移能力,诱导细胞分化;(5)p-P38蛋白水平明显升高(P<0.01),而p-ERK、P-SPKA/JNK蛋白水平明显降低(P<0.01)。结论:CMSP抑制食管癌TE-13细胞的增殖、诱导其分化,其作用机制可能与上调MAPK信号通路中P-P38和下调P-ERK、P-SPKA/JNK有关。

PI-88对TE-13细胞及裸鼠移植瘤中乙酰肝素酶表达的影响

目的探讨硫酸化寡聚多糖(PI-88)对食管鳞癌细胞株TE-13乙酰肝素酶(Hpa)表达的影响,以及对裸鼠人食管癌移植瘤生长、血管生成及Hpa蛋白表达的影响。方法体外培养TE-13细胞,实验分为A组(对照组)、B组(15 mg/L PI-88干预组)和C组(30 mg/L PI-88干预组)。培养36 h后Western blot检测各组细胞Hpa蛋白表达。选取10只BALB/c/nu裸鼠,皮下接种TE-13细胞建立食管癌裸鼠移植瘤模型,建模成功后随机均分为观察组及对照组。观察组腹腔注射PI-88 40 mg/(kg·d),对照组给予等剂量生理盐水,连续注射14 d。每2 d测量移植瘤体积,注射第14天处死动物,剥除移植瘤行CD34染色,检测微血管密度(MVD)。Western blot及免疫组化染色检测Hpa蛋白表达。结果与A组相比,B、C组细胞Hpa蛋白表达量明显降低(P<0.001),且存在药物浓度依赖性。观察组裸鼠移植瘤体积、MVD值、Hpa蛋白表达水平及阳性细胞数均低于对照组(均P<0.05)。结论 PI-88可抑制TE-13细胞及食管癌裸鼠皮下移植瘤中Hpa表达,并抑制肿瘤生长和血管生成。

香加皮水提取物诱导人食管癌细胞TE-13凋亡的实验研究

[目的]运用多种技术手段研究香加皮水提取物诱导人食管癌细胞TE-13凋亡。[方法]利用MTT染色在普通光镜下观察细胞凋亡形态学变化并观测药物对肿瘤细胞的抑制率;通过流式细胞仪分析人食管癌TE-13细胞凋亡率、细胞周期变化;DNA琼脂糖凝胶电泳方法检测肿瘤细胞凋亡的DNA水平变化;激光扫描共聚焦显微镜(LSCM)检测细胞内钙离子浓度变化。[结果]经香加皮水提取物处理的人食管癌细胞TE-13出现核固缩、凋亡小体、新月状浓染区等细胞凋亡形态学改变,各剂量药物处理组的肿瘤细胞均表现生长抑制,且具有剂量依赖性,250μg/ml香加皮水提取物处理组的抑制率达91.02%。DNA琼脂糖凝胶电泳呈现典型的梯形电泳条带。药物处理组的肿瘤细胞更多地被阻止于G2/M期,各剂量组均出现明显的凋亡变化,最大凋亡率可达20.3%。各剂量药物处理组的肿瘤细胞内的Ca2+浓度明显高于对照组(P<0.01)。[结论]香加皮水提取物可明显抑制人食管癌细胞TE-13的生长增殖,诱导细胞凋亡,并能改变该肿瘤细胞周期分布,阻止细胞周期于G2/M期。

食管鳞状细胞癌TE-13细胞线粒体DNA及细胞凋亡检测

目的:检测人食管鳞状细胞癌TE-13细胞中线粒体DNA(mtDNA)与细胞凋亡的发生情况及可能的关系。方法:TE-13细胞分为2组:溴化乙啶(EB)处理组在细胞培养液中加入50mg/LEB,未处理组常规培养;在培养第4、8和12天分别利用半定量RT-PCR检测2组细胞mtDNA的表达,利用流式细胞术检测细胞的凋亡情况。结果:EB处理组的第4天和第8天mtDNA的表达量分别为(0.467±0.031)和(0.197±0.015),到第12天mtDNA已完全丢失,未处理组分别为(0.660±0.046)、(0.673±0.031)和(0.653±0.021),差异有统计学意义(F组间=1133.878,F时间=109.058,F交互=104.597;P<0.001)。流式细胞术检测结果显示,EB处理组凋亡细胞百分比高于未处理组(F组间=2773.035,F时间=407.652,F交互=406.641;P<0.001)。结论:抑制TE-13细胞中mtDNA的复制可能会促进细胞凋亡。

环状RNA circ-Foxo3模拟物转染对人食管癌细胞株TE-13增殖、凋亡、放射敏感性的影响

目的观察环状RNA circ-Foxo3模拟物(circ-Foxo3 mimics)对人食管鳞癌细胞株TE-13增殖、凋亡、放射敏感性的影响,并探讨其机制。方法体外培养人食管鳞癌细胞株TE-13,将circ-Foxo3 mimics和NC转染至TE-13细胞中培养(分别计为过表达组、NC组)。采用qRT-PCR法检测TE-13细胞circ-Foxo3,CCK8实验检测两组细胞OD值,流式细胞术检测两组细胞凋亡率,克隆形成实验检测两组细胞放射敏感性;Western blotting法检测两组细胞PTEN蛋白。结果 TE-13细胞转染前后circ-Foxo3相对表达量分别为0. 05±0. 01、3. 99±0. 17,转染前后比较,P<0. 05。过表达组0、24、48、72、96 h OD值分别为0. 20±0. 00、0. 32±0. 02、0. 46±0. 03、0. 74±0. 02、1. 26±0. 01,NC组分别为0. 20±0. 00、0. 45±0. 03、0. 72±0. 02、1. 35±0. 03、2. 18±0. 01,两组比较(除0 h外),P均<0. 05。过表达组照射前后细胞凋亡率分别为4. 83±0. 85、11. 67±0. 47,NC组分别为0. 37±0. 06、5. 17±0. 25,两组同组照射前后及两组治疗后比较,P均<0. 05。过表达组0、2、4、6、8 Gy细胞存活分数分别为0. 20±0. 00、0. 83±0. 04、0. 67±0. 01、0. 50±0. 03、0. 31±0. 01,NC组分别为0. 20±0. 00、0. 91±0. 02、0. 84±0. 01、0. 65±0. 02、0. 52±0. 02,两组比较(除0 Gy外),P均<0. 05。过表达组照射前后PTEN蛋白条带灰度值分别为0. 71±0. 02、0. 87±0. 01,NC组分别为0. 53±0. 04、0. 55±0. 04,两组同组照射前后及两组治疗后比较,P均<0. 05。结论 circ-Foxo3mimics转染能抑制细胞增殖,促进凋亡,增加了细胞对放射的敏感性,机制可能与circ-Foxo3上调PTEN蛋白表达有关。

乳腺癌患者病理特征与Bcl-2、CXCL13、PAX8表达情况的关系分析

目的分析乳腺癌患者病理特征与B细胞淋巴瘤/白血病-2基因(Bcl-2)、趋化因子配体13(CXCL13)、配对盒基因8抗体(PAX8)表达情况的关系。方法收集2021年1月至2023年1月该院收治的160例乳腺癌患者临床资料。采用免疫组化法对其癌组织与癌旁组织Bcl-2、CXCL13、PAX8表达情况进行检测,并分析3项指标与患者病理特征的关系。结果与癌旁组织比较,癌组织Bcl-2、CXCL13、PAX8阳性率更高,差异有统计学意义(P<0.05)。与雌激素受体(ER)阴性、肿瘤最大径≥3 cm、孕激素受体(PR)阴性患者比较,ER阳性、肿瘤最大径<3 cm、PR阳性患者中Bcl-2高表达占比更高,差异有统计学意义(P<0.05);与无淋巴结转移、Ⅰ~Ⅱ期患者比较,淋巴结转移、Ⅲ~Ⅳ期患者中CXCL13高表达占比更高,差异有统计学意义(P<0.05);与Ⅰ~Ⅱ期、高/中分化、无淋巴结转移患者比较,Ⅲ~Ⅳ期、低分化、有淋巴结转移患者中PAX8高表达占比更高,差异有统计学意义(P<0.05)。ER、PR表达情况与Bcl-2表达情况呈正相关(P<0.05),肿瘤最大径与Bcl-2表达情况呈负相关(P<0.05);临床分期、淋巴结转移情况与CXCL13、PAX8表达情况呈正相关(P<0.05);分化程度与PAX8表达情况呈负相关(P<0.05)。结论乳腺癌患者Bcl-2、CXCL13、PAX8表达情况对疾病的发生和发展具有明显影响,有望成为评估乳腺癌患者病情严重程度的标志物。

血清胸腺活化调节趋化因子、CXC亚家族趋化因子13与弥漫大B细胞淋巴瘤患者化疗疗效和预后的关系研究

目的探讨血清胸腺活化调节趋化因子(TARC)、CXC亚家族趋化因子13(CXCL13)与弥漫大B细胞淋巴瘤(DLBCL)患者化疗疗效和预后的关系。方法选取2017年1月至2020年6月该院收治的285例DLBCL患者(DLBCL组)及同期健康体检者160例(对照组)作为研究对象,DLBCL患者接受利妥昔单抗+环磷酰胺+多柔比星+长春新碱+泼尼松(R-CHOP)相关化疗方案,根据化疗效果分为有效组和无效组。比较DLBCL组与对照组、有效组与无效组血清TARC、CXCL13水平;随访统计DLBCL患者3年总生存期(OS)及无进展生存期(PFS),采用Logistic回归分析DLBCL患者预后及疾病进展的影响因素,并构建回归预测模型,采用受试者工作特征(ROC)曲线分析其预测评估效能。采用Kaplan-Meier生存曲线分析不同水平血清TARC、CXCL13与DLBCL患者3年OS及PFS的关系。结果DLBCL组治疗前血清TARC、CXCL13水平高于对照组(P<0.05)。DLBCL患者化疗有效率为85.26%,无效组治疗前血清TARC、CXCL13水平高于有效组(P<0.05)。多因素Logistic分析结果显示,Ann Arbor分期Ⅲ/Ⅳ期、TARC高表达及CXCL13高表达均是DLBCL患者预后的独立危险因素(P<0.05)。乳酸脱氢酶水平升高、TARC高表达及CXCL13高表达均是DLBCL患者疾病进展的独立危险因素(P<0.05)。以上述影响因素构建回归预测模型,ROC曲线分析显示,预测模型预测预后的曲线下面积(AUC)为0.874,预测疾病进展的AUC为0.911。TARC低表达患者的3年OS、PFS优于高表达患者(P<0.05),CXCL13低表达患者的3年OS、PFS优于高表达患者(P<0.05)。结论DLBCL患者血清TARC、CXCL13水平异常升高,血清TARC、CXCL13低表达的DLBCL患者具有更好的化疗效果及预后。包括血清TARC、CXCL13在内的多因子预测模型对DLBCL患者预后具有较高的评估效能。

血清sCD40L、ADAMTS13与老年髋部骨折患者术后下肢深静脉血栓形成的关系

目的 探讨血清可溶性细胞表面分化抗原40配体(sCD40L)、血管性血友病因子裂解蛋白酶13(ADAMTS13)水平与老年髋部骨折患者术后下肢深静脉血栓(DVT)形成的关系。方法 选取2022年6月至2023年6月在该院就诊的192例老年髋部骨折患者,根据其术后是否发生下肢DVT分为非DVT组(120例)和DVT组(72例)。酶联免疫吸附试验检测各组血清sCD40L、ADAMTS13水平;Pearson法分析患者血清sCD40L与ADAMTS13水平的相关性;多因素Logistic回归模型分析影响老年髋部骨折患者术后发生下肢DVT的因素;受试者工作特征(ROC)曲线评估血清sCD40L、ADAMTS13水平对老年髋部骨折患者术后发生下肢DVT的预测价值。结果 两组高脂血症占比及骨折至开始手术时间比较,差异有统计学意义(P<0.05)。与非DVT组比较,DVT组血清sCD40L水平升高(P<0.05),ADAMTS13水平降低(P<0.05);Pearson法分析结果显示,患者血清sCD40L水平与ADAMTS13水平呈负相关(r=-0.457,P<0.001);多因素Logistic回归模型分析结果显示,高脂血症、骨折至开始手术时间长、血清sCD40L水平升高是老年髋部骨折患者术后发生下肢DVT的危险因素(P<0.05);血清ADAMTS13水平升高是影响老年髋部骨折患者术后发生下肢DVT的保护因素(P<0.05)。血清sCD40L、ADAMTS13联合预测老年髋部骨折患者术后发生下肢DVT的曲线下面积为0.812,大于sCD40L和ADAMTS13单独预测(P<0.05)。结论 老年髋部骨折术后发生下肢DVT患者血清sCD40L水平升高,ADAMTS13水平降低,二者水平可反映DVT的发生风险,且对老年髋部骨折患者发生下肢DVT具有一定的预测价值。

Interleukin-13 inhibits cytokines synthesis by blocking nuclear factor-κB and c-Jun N-terminal kinase in human mesangial cells

Objective： Monocytes/macrophages, proinflammatory cytokines and chemokines are important in the pathogenesis of glomerulonephritis. Interleukin （IL） -13 has been shown to exert potent anti-inflammatory properties. This study was designed to investigate the effect of IL-13 on the expression of proinflammatory cytokines, chemokines and profibrogenic cytokines and the involved molecular mechanism in cultured human mesangial cells （HMCs）. Methods： The expressions of proinflammatory cytokines, chemokines and profibrogenic cytokines were determined by ribonuclease protection assay （RPA）. Activity of nuclear factor-kappa B （NF-κB） and activa- tor protein-1 （AP-1） was examined by electrophoretic mobility shift assay （EMSA）. NF-κB subunit p65 nuclear transportation and c-Jun N-terminal kinase （JNK） activity were assayed by immunoblot. Results： Recombinant IL-13 inhibited tumor necrosis factor-α （TNF-u）, IL-1α, IL-1β, monocyte chemoattractant protein-1 （MCP-1）, IL-8, and transforming growth factor-β1 （TGF-β1） mRNA expressions in a dose-dependent manner. Lipopoly- sacchorides （LPS） dramatically increased NF-κB DNA binding activity of HMCs, which was inhibited by IL-13 in a dose-dependent manner. LPS-activated NF-κB contained p50 and p65 dimers, but not c-Rel subunit. IL-13 blocked LPS-induced NF-κB subunit p65. LPS stimulated JNK/AP-1 activation, which was inhibited by IL-13 in a dose-dependent manner. Conclusion： IL-13 inhibits proinflammatory cytokines, chemokines, and profibrogenic cytokines synthesis by blocking NF-κB and JNK/AP-1 activation. These observations point to the importance of IL-13 in the modulation of inflammatory processes in the renal glomerulus.

Construction of eukaryotic expression vector of human S100A13 gene and its effect on proliferation of human thyroid cancer cell line TT

Objective To investigate the effect of exogenous S100A13 gene overexpression on the proliferation of human thyroid cancer cell line TT.Methods The recombinant ORF of S100A13 tagged with six histidines at the 5' end was subcloned into the pcDNA3.2/V5/GW/D-TOPO vector and sequenced.The eukaryotic expression plasmid pcDNA3.2/V5 /GW/D-S100A13 and empty vector pcDNA3.2/V5/GW/D were transfected into TT cells.The positive clones were selected by G418.The expressions of S100A13 mRNA and protein were detected by real time reverse transcription-polymerase chain reaction(RT-PCR) and Western blot.The effect of S100A13 on cell proliferation and cell cycle was evaluated by cell growth curve,MTT colorimetric assay and flow cytometry.Results S100A13 gene tagged with six histidines at the 5 ' end was confirmed to be inserted into the pcDNA3.2/V5/GW/D vector correctly.TT-S100A13-V5 cells,which over-expressed S100A13,were constructed successfully.TT-S100A13-V5 cells grew much faster than TT-V5 and TT cells(P <0.001).The proportions of both S and G2/M phase cells were significantly higher in TT-S100A13-V5 cells than those in TT-V5 and TT cells(P <0.001).Conclusion The eukaryotic expression vector containing human S100A13 gene has been successfully constructed,which highly expresses S100A13 in TT cells.Exogenous S100A13 gene overexpression accelerates TT cell proliferation and drives the cell cycle progression of TT cells from G0/G1 phase to S and G2/M phases.

IL-13Ra2-and glioma stem cell-pulsed dendritic cells induce glioma cell death in vitro

Objective Gliomas are the most common malignant tumors in the central nervous system.Despite multiple therapies including surgery,chemotherapy,and radiotherapy,the prognosis of patients remains poor.Immunotherapy is an alternative method of treating glioma,and the use of dendritic cell vaccines is one of the promising treatment options.However,there is no specific tumor cell antigen that can trigger dendritic cells(DCs).IL-13Ra2 is a specific antigen expressed in glioma cells;in the current study,we have attempted to explore whether IL-13Ra2 could be the antigen that triggers DCs and to envisage its application as potential therapy for glioma.Methods The expression of IL-13Ra2 was detected in U251 glioma cell lines and primary glioma tissues using different methods.DCs from human blood were isolated and pulsed with recombinant IL-13Ra2,following which the cytotoxicity of these DCs on glioma cells was detected and analyzed.Results About 55.9% human glioma tissue cells expressed IL-13Ra2,while normal brain tissue cells did not show any expression.DC vaccines loaded with IL-13Ra2,glioma cell antigen,and brain tumor stem cell(BTSC) antigen could significantly stimulate the proliferation of T lymphocytes and induce cell death in the glioma tissue.Compared to other groups,DC vaccines loaded with BTSC antigen showed the strongest ability to activate cytotoxic T lymphocytes(CTLs),while the glioma cell antigen group showed no significant difference.Conclusion IL-13Ra2,which is expressed in gliomas and by glioma stem cells,as well as IL-13Ra2 could prove to be potential antigens for DC vaccine-based immunotherapy.

Tinospora crispa extract inhibits MMP-13 and migration of head and neck squamous cell carcinoma cell lines

Objective: To investigate the effect of Tinospora crispa(T. crispa) extract on matrix metalloproteinase 13(MMP-13) expression and cell migration. Methods: The cytotoxicity of T. crispa extract was examined by 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide assay on head and neck squamous cell carcinoma(HNSCC) cell lines. The effect on expression of MMP-13 was analysed by RT-PCR and ELISA. The migration was assessed by wound healing assay. Results: MMP-13 m RNA was highly expressed in the metastatic human HNSCC cell lines, HN22 and HSC-3. T. crispa extract at a concentration of 100.0 μg/m L caused about 50% reduction of cell survival. T. crispa extract at a non-toxic concentration of 12.5, 25.0 and 50.0 μg/m L signii cantly suppressed MMP-13 m RNA expression and secreted MMP-13 in both HN22 and HSC-3. The expression of tissue inhibitors of metalloprotease by HSC-3 cells was attenuated by 25.0 and 50.0 μg/m L of T. crispa extract. Addition of the extract to cells in a wound healing assay showed inhibition of cell migration by HN22 cells. Conclusions: These data suggest that T. crispa could be considered as a potential therapeutic drug to prevent metastasis of HNSCC.

Glycosylation-independent binding to extracellular domains 11-13 of mannose-6-phosphate/insulin-like growth factor-2 receptor mediates the effects of soluble CREG on the phenotypic proliferation of vascular smooth muscle cells

Background The present study aimed to investigate the detailed mode and specific sites for their binding as well as the functional relevance of this binding in the phenotypic proliferation of vascular smooth muscle cells(SMCs). Methods CREG knocked-down SMCs were employed to evaluate the biological activity of wtCREG and mCREG.Expressions of SMC differentiation markers SM myosin heavy chain(SM-MHC),SM-actin,heavy caldesmon and myocardin were determined by Western blotting using specific antibodies. Cellular growth of SMCs was assessed by bromide dewuridine (BrdU) incorporation and cell cycle analysis on fluorescence-activated cell sorting(FACS).A solid-phase binding assay was used to study the binding of CREG to extracellular domains of M6P/IGF2R.The cellular co-localization of the two recombinant CREGs with M6P/IGF2R was detected on SMC surface by immunoprecipitation and immunofluorescence analysis.Results The molecular weight of wtCREG was around 30 kD while that of the mCREG was～25 kD.Treatment of wtCREG with PNGase F reduced its molecular weight from～30 kD to～25 kD,whereas PNGase F treatment had no effect on the molecular weight of mCREG.Both wtCREG and mCREG proteins enhanced SMC differentiation,inhibited BrdU incorporation,and arrested cell cycle progression when added to the culture medium.In CREG knocked-down SMCs,the amount of CREG detected by immunoblotting in M6P/IGF2R immunoprecipitates was significantly reduced when compared to normal cells.Both recombinant CREGs co-immunoprecipitated with M6P/IGF2R, although slightly reduced amount of the mutant CREG was detected in M6P/IGF2R immunoprecipitates.Immunostaining revealed that His-tagged CREGs co-localized with IGF2R on the cell surface in a glycosylation-independent manner.In vitro binding assay showed that CREGs bound to M6P/ IGF2R extracellular domains 7-10 and 11-13 in a glycosylation -dependent and -independent manner,respectively.Further blocking experiments using soluble M6P/IGF2R fragments and M6P/IGF2R neutralizing antibody indicated that the biological activities of recombinant CREGs in SMC growth and the up-regulation of SMC differentiation markers were all abolished by treatment with the M6P/IGF2R neutralizing antibody. However,although the growth inhibitory effect of wtCREG was nearly abolished by D7-10 or D11-13,the effect of mCREG was only reversed by Dll-13,indicating that the binding to domains 11-13 is required for CREG to modulate the proliferation of SMCs.Conclusions These data suggest that solubleCREG proteins can exert their biological function via binding to the extracellular domains 7-10 and 11-13 of cell surface M6P/IGF2R in both a glycosylation-dependent and -independent manner.

Regulation of mitochondrial carrier SLC25A13 on breast cancer cell cycle in vitro

Objective·To investigate the role of mitochondrial solute carrier family 25 member 13(SLC25A13)on breast cancer development.Methods·SLC25A13 mRNA and protein expressions in invasive breast cancer tissues and normal breast tissues were from The Cancer Genome Atlas(TCGA)breast cancer dataset.Survival analysis was conducted online by Kaplan-Meier software.MCF-7 cell line was used for in vitro cell assay.Knockdown of SLC25A13 and sirtuin 2(SIRT2)were conducted by siRNA transfection.Cell viability was measured with trypan blue exclusion.Cell cycle arrest was determined by flow cytometry.The mRNA expression of SLC25A13 and P27 were detected by quantitative PCR.The protein level of SLC25A13,P27 and SIRT2 were detected by Western blotting.Protein half-life of P27 was assessed by Western blotting after cycloheximide treatment.Results·SLC25A13 was up-regulated in invasive breast cancer tissues.High expression of SLC25A13 correlated with poor overall survival and breast cancer recurrence.SLC25A13 knockdown inhibited MCF-7 cell cycle progression.P27 and SIRT2 both accumulated after SLC25A13 knockdown.P27 accumulation resulted from prolonged protein half-life.Knockdown of SIRT2 restored cell cycle arrest as well as P27 accumulation caused by SLC25A13 silencing.Conclusion·High expression of SLC25A13 may promote cell cycle progression via SIRT2 in breast cancer development.

ILC2和MDSC及其相关细胞因子IL-13和iNOS在宫颈癌中的表达及其列线图模型的构建和评价

目的:研究2型固有淋巴样细胞(ILC2)和髓源性抑制细胞(MDSC)及其相关细胞因子IL-13和诱导型一氧化氮合酶(iNOS)在宫颈癌(CC)中的表达,并基于其构建CC发病风险的列线图预测模型。方法:采集2022年5月至2024年1月在新疆医科大学第一附属医院手术切除的40例CC组织及100例外周血作为CC组,选取同期收治的30例子宫肌瘤经CC筛查为阴性的宫颈组织和100例正常健康个体外周血作为对照组。用多重免疫荧光技术(mIF)及免疫组化染色(IHC)法检测两组组织中ILC2和MDSC细胞浸润及其相关细胞因IL-13和iNOS的表达;使用流式细胞术和ELISA技术分别检测两组外周血中ILC2和MDSC及IL-13和iNOS的表达差异;通过Person相关性分析评估其相关性;使用单因素和多因素Logistic分析来确定ILC2和MDSC及IL-13和iNOS是否为CC发病的独立危险因素,再利用R软件建立免疫预测模型,使用ROC曲线下面积(AUC值)、Hosmer-Lemeshow检验、校准曲线、临床决策曲线和临床影响曲线来分别评估模型。结果:CC组中ILC2及MDSC及其相关细胞因子IL-13和iNOS均高于对照组(均P<0.05),且其均呈正相关(均P<0.05);经过单因素及多因素Logistic回归分析显示,ILC2、MDSC及IL-13、iNOS均是CC发病的独立危险因素(均P<0.05);基于这些危险因素的CC发病列线图,经过验证提示,该列线图模型具有一定的临床实用价值。结论:ILC2和MDSC及其相关的细胞因子IL-13和iNOS在CC组织及外周血中均呈高表达,基于这些危险因素构建的预测模型具有良好的预测能力和一定的实用性,为CC的早期诊断和治疗提供了一种简便有效的辅助工具。

Two potentially specific but relevant patterns of proteomic change Response of SH-SY5Y cells to differentiation with retinoic acid followed by phorbol ester 12-O-tetradecanoyl-phorbol-13-acetate, and susceptibility of differentiated cells to dopamine

Dopamine （DA） exposure at a dose of 100 pmol/L for 24 hours causes oxidative stress in SH-SY5Y cells with induction of neuronal differentiation by retinoic acid （RA,10 pmol/L,72 hours） followed by phorbol ester 12-O-tetradecanoyl-phorbol-13-acetate （TPA,80 nmol/L,72 hours）. However,it remains unclear whether the alteration of phenotype observed in response to oxidative stress is associated with protein regulation in this cellular model for Parkinson＇s disease. The present study detected protein regulation affected by oxidative stress at a proteomic level：selection of differentially altered proteins using two dimensional difference in-gel electrophoresis and identification of these proteins using matrix assisted laser desorption/ionization time-of-flight mass spectrometry. The results demonstrated significant alterations in expression of six proteins in SH-SY5Y cells following the differentiation and fourteen proteins in the differentiated cells following the exposure,exemplified by an increase of tubulin alpha1 in the former but a decrease of tubulin alpha-ubiquitous chain in the latter. These results suggest that two potentially specific but relevant patterns of proteomic change may be produced in SH-SY5Y cells with the induction of differentiation by RA followed by TPA,and in the differentiated cells after DA exposure.

Replication of M13 single-stranded DNA bearing a sitespecific ethenocytosine lesion by Escherichia coil cell extracts

Previous investigation on the mutagenic effects of 3,N4-Ethenocytosine (εC), a nonpairing DNA lesion,revealed the existence of a novel SOS-independent inducible mutagenic mechanism in E. coli termed UVM for UV modulation of mutagenesis. To investigate whether UVM is mediated by an alteration of DNA replication, we have set up an in vitro replication system ill which phage M13 viral single-stranded DNA bearing a single site-specific (εC) residue is replicated by soluble protein extracts from E. coli cells. Replication products were analyzed by agarose gel electrophoresis and the frequency of translesion synthesis was determined by restriction endonuclease analyses. Our data indicate that DNA replication is strongly inhibited by εC, but that translesion DNA synthesis does occur in about 14% of the replicated DNA molecules. These results are very similar to those observed previously in vivo, and suggest that this experimental system may be suitable for evaluating alterations in DNA replication in UVM-induced cells.