Upregulation of stromal cell-derived factor-1 alpha/CXCR4 axis-induced migration of human neural progenitors by tumor necrosis factor-alpha and interleukin-8

BACKGROUND： Studies of several animal models of central nervous system diseases have shown that neural progenitor cells （NPCs） can migrate to injured tissues. Stromal cell-derived factor 1 alpha （SDF-la）, and its primary physiological receptor CXCR4, have been shown to contribute to this process. OBJECTIVE： To investigate migration efficacy of human NPCs toward a SDF-1α gradient, and the regulatory roles of tumor necrosis factor-α （TNF-α） and interleukin-8 （IL-8） in SDF-1α/CXCR4 axis-induced migration of NPCs. DESIGN, TIME AND SETTING： An in vitro, randomized, controlled, cellular and molecular biology study was performed at the Laboratory of Department of Cell Biology, Medical College of Soochow University between October 2005 and November 2007. MATERIALS： SDF-1α and mouse anti-human CXCR4 fusion antibody were purchased from R＆D Systems, USA. TNF-αwas purchased from Biomyx Technology, USA and IL-8 was kindly provided by the Biotechnology Research Institute of Soochow University. METHODS： NPCs isolated from forebrain tissue of 9 to 10-week-old human fetuses were cultured in vitro. The cells were incubated with 0, 20, and 40 ng/mL TNF-α, or 0, 20, and 40 ng/mL IL-8, for 48 hours prior to migration assay. For antibody-blocking experiments, cells were further pretreated with 0, 20, and 40 μg/mL mouse anti-human CXCR4 fusion antibody for 2 hours. Subsequently, the transwell assay and CXCR4 blockade experiments were performed to evaluate migration of human NPCs toward a SDF-1α gradient. Serum-free culture medium without SDF-1α served as the negative control. MAIN OUTCOME MEASURES： The transwell assay was performed to evaluate migration of human NPCs toward a SDF-1α gradient, which was blocked by fusion antibody against CXCR4. In addition, CXCR4 expression in human NPCs stimulated by TNF-α and IL-8 was measured by flow cytometry. RESULTS： Results from the transwell assay demonstrated that SDF-1α was a strong chemoattractant for human NPCs （P 〈 0.01）, and 20 ng/mL produced the highest levels of migration. Anti-human CXCR4 fusion antibody significantly blocked the chemotactic effect （P 〈 0.05）. Flow cytometry results showed that treatment with TNF-α and IL-8 resulted in increased CXCR4 expression and greater chemotaxis efficiency of NPCs towards SDF-1α（P 〈 0.01）. CONCLUSION： These results demonstrated that SDF-la significantly attracted NPCs in vitro, and neutralizing anti-CXCR4 antibody could block part of this chemotactic function. TNF-α and IL-8 increased chemotaxis efficiency of NPCs towards the SDF-1αgradient by upregulating CXCR4 expression in NPCs.

玻璃体腔注射雷珠单抗对增殖性糖尿病性视网膜病变患者视力及血清GAS6、SDF-1及VEGF的影响

目的 探讨增殖性糖尿病视网膜病变(PDR)给予玻璃体腔注射雷珠单抗药物对患者视力以及血清人生长停滞特异性蛋白(GAS6)、人基质细胞衍生因子1(SDF-1)、血管内皮细胞生长因子(VEGF)影响。方法 纳入2022年1月至12月收治的PDR患者82例,按照随机数字表法分为观察组和对照组,每组41例。对照组采用玻璃体切割术(PPV)治疗,观察组采用联合玻璃体切割术(PPV)术前经玻璃体腔注射雷珠单抗治疗。对比2组的治疗效果,2组患者术前与术后1周的视力以及眼压水平,2组患者术前与术后1周血清GAS6、SDF-1、VEGF水平变化,2组术后并发症发生情况。结果 观察组治疗总有效率为95.12%高于对照组的78.05%(P<0.05)。2组患者术后1周的眼压、血清GAS6、SDF-1、VEGF水平均较术前降低,且观察组术后1周的上述指标水平低于对照组(P<0.05)。2组术后1周视力较术前升高,且观察组视力水平高于对照组(P<0.05)。观察组患者术后并发症总发生率为4.88%低于对照组的24.39%(P<0.05)。结论 应用玻璃体腔注射雷珠单抗辅助PPV治疗PDR,效果满意,可显著提高患者视力,降低眼压,降低血清GAS6、SDF-1、VEGF水平,且术后并发症发生率低,值得推广。

西格列汀激活基质细胞衍生因子-1/CXC趋化因子受体4信号通路对脂多糖诱导的人牙周膜干细胞增殖、凋亡、炎症和成骨分化的影响

目的 探讨西格列汀对脂多糖(LPS)诱导的炎症微环境下人牙周膜干细胞(hPDLSCs)增殖、凋亡、炎症和成骨分化的影响及分子机制。方法 体外培养hPDLSCs,用不同浓度的西格列汀处理后检测细胞活力,以确定后续西格列汀实验浓度。采用1μg/mL LPS刺激诱导24 h建立hPDLSCs炎症模型并分为空白组、对照组、西格列汀低浓度组(0.5μmol/L)、西格列汀中浓度组(1μmol/L)、西格列汀高浓度组(2μmol/L)、西格列汀高浓度+基质细胞衍生因子-1 (SDF-1)/CXC趋化因子受体4 (CXCR4)通路抑制剂(AMD3100)组(2μmol/L+10μg/mL)。细胞计数试剂盒-8检测培养24、48、72 h后的hPDLSCs增殖活性;流式细胞术检测培养72 h后hPDLSCs凋亡情况;诱导成骨分化21 d后茜素红染色检测hPDLSCs成骨分化能力,试剂盒测定hPDLSCs中碱性磷酸酶(ALP)活性;酶联免疫吸附检测hPDLSCs培养上清液中炎症因子肿瘤坏死因子(TNF)-α、白细胞介素(IL)-1β、IL-6水平;实时荧光定量聚合酶链反应(RT-qPCR)检测hPDLSCs中成骨分化相关基因Runt相关转录因子2 (RUNX2)、骨钙素(OCN)、骨桥蛋白(OPN)及SDF-1和CXCR4 mRNA表达;Western blot检测hPDLSCs中SDF-1、CXCR4蛋白表达。结果 与空白组比较,对照组hPDLSCs增殖活性、矿化结节数量、染色强度、ALP活性和RUNX2、OCN、OPN mRNA及SDF-1、CXCR4 mRNA和蛋白表达水平显著降低,凋亡率、TNF-α、IL-1β、IL-6水平显著升高(P<0.05);与对照组比较,西格列汀低、中、高浓度组hPDLSCs增殖活性、矿化结节数量、染色强度、ALP活性和RUNX2、OCN、OPN mRNA及SDF-1、CXCR4 mRNA和蛋白表达水平依次升高,凋亡率、TNF-α、IL-1β、IL-6水平依次降低(P<0.05);AMD3100可部分逆转高浓度西格列汀对LPS诱导的hPDLSCs的作用效果(P<0.05)。结论 西格列汀可能通过激活SDF-1/CXCR4信号通路促进LPS诱导的炎症微环境下hPDLSCs的增殖和成骨分化,抑制hPDLSCs凋亡和炎症反应。

Prognostic role of the stromal cell derived factor-1 in patients with hepatitis B virus-related acute-on-chronic liver failure

BACKGROUND Stromal cell derived factor-1(SDF-1)plays a pivotal role in the recruitment of stem cells to injured livers.However,the changes of SDF-l in patients with hepatitis B virus(HBV)-related acute-on-chronic liver failure(ACLF)have yet to be elucidated.AIM To study the SDF-1 changes in patients with HBV-related ACLF.METHODS 30 patients with HBV-related ACLF,27 patients with chronic hepatitis B and 20 healthy individuals are involved in our study.The SDF-l mRNA expression in liver tissue was detected by quantitative real-time polymerase chain reaction.Immunohistochemical staining was performed to illustrate the expression of SDFl,CXC receptor 4(CXCR4)and Ki67.The serum SDF-l concentrations were also detected by enzyme-linked immunosorbent assays.RESULTS The expression of SDF-1 mRNA from ACLF patients was remarkably higher than that from other patients(both P<0.05).The expression of SDF-l,CXCR4 and Ki67 from ACLF were the highest among the three groups(all P<0.01).The serum SDF-l levels in ACLF patients were significantly lower than that in other patients(both P<0.01).Moreover,in ACLF patients,the serum SDF-1 Levels were positively correlated with serum total bilirubin and international normalized ratio.In addition,the serum SDF-l levels in survival were significantly lower compared with the non-survivals(P<0.05).The area under the curve for the serum SDF-1 level in predicting 28-d mortality was 0.722(P<0.05).CONCLUSION This study provides the SDF-1 changes in patients with HBV-related ACLF.The SDF-1 Level at admission may serve as a promising prognostic marker for predicting short-term prognosis.

SDF-1/CXCR4 expression in bladder cancer tissue and the correlation with negative costimulatory molecule PD-L1, cell apoptosis and invasion

Objective:To study the SDF-1/CXCR4 expression in bladder cancer tissue and the correlation with negative costimulatory molecule PD-L1, cell apoptosis and invasion.Methods: A total of 118 cases of bladder cancer tissue and para-carcinoma tissue surgically removed in our hospital between May 2014 and May 2016 were selected as the research samples, the RNA was extracted and then reverse-transcribed into cDNA, and the expression levels of SDF-1/CXCR4, PD-L1/PD-1, cell apoptosis-related molecules and cell invasion-related molecules were detected.Results: SDF-1 and CXCR4 mRNA expression in bladder cancer tissue were significantly higher than those in para-carcinoma tissue;PD-L1, PD-1, Rec1, Survivin, MRPS5, Nanog, BCAPP2Ac, TRPM8, TRPV2, ILK,β-catenin and GUGBP1 mRNA expression in bladder cancer tissue were significantly higher than those in para-carcinoma tissue and positively correlated with SDF-1 and CXCR4 mRNA expression.Conclusion:Highly expressed SDF-1/CXCR4 in bladder cancer tissue are closely related to the high expression of negative costimulatory molecule PD-L1, pro-proliferation molecules and pro-invasion molecules, and SDF-1/CXCR4 can promote the immune escape, proliferation and invasion of bladder cancer cells.

SDF-1通过PI3K/Akt和MAPK/Erk信号通路对人微血管内皮细胞功能产生影响

目的 :观察基质细胞衍生因子-1(stromal cell derived factor-1,SDF-1)对人微血管内皮细胞(human microvascular endothelial cell line-1,HMEC-1)功能的影响,并对相关机制进行初步探讨,从而明确SDF-1在糖尿病血管病变中的作用。方法:体外培养HMEC-1,分别在培养基中加入不同浓度的SDF-1(0、25、50、100μg/L),Western blot检测HMEC-1中PI3K/Akt和MAPK/Erk信号通路的活化情况,MTT和流式细胞分析检测HMEC-1增殖和凋亡能力的变化情况,划痕愈合实验检测HMEC-1迁移能力的变化情况。采用PI3K/Akt和MAPK/Erk信号通路抑制剂LY294002和U0126阻断HMEC-1中PI3K/Akt和MAPK/Erk信号通路后,再以SDF-1处理HMEC-1,MTT和流式细胞分析检测HMEC-1增殖和凋亡能力的变化情况;划痕愈合实验检测HMEC-1迁移能力的变化情况。结果:Western blot结果显示,25μg/L的SDF-1处理即可显著活化HMEC-1中的PI3K/Akt和MAPK/Erk信号通路,且随着SDF-1处理浓度的升高,PI3K/Akt和MAPK/Erk信号通路活化水平逐渐升高。同0μg/L的SDF-1处理组相比,25、50、100μg/L的SDF-1均可显著加强HMEC-1的增殖和迁移能力(P<0.01),并抑制HMEC-1的凋亡水平(P<0.01),且这种作用具有剂量依赖性。当采用LY294002和U0126阻断HMEC-1中的PI3K/Akt和MAPK/Erk信号通路后,SDF-1促HMEC-1增殖和迁移能力及抑制HMEC-1凋亡的能力均显著降低(P<0.01)。结论:SDF-1可通过活化PI3K/Akt和MAPK/Erk信号通路,进而促进HMEC-1的增殖和迁移,并抑制HMEC-1的凋亡水平,从而在糖尿病血管病变中发挥一定的作用。

SDF-1-pIRES2-EGFP真核表达载体的构建

目的从ATCC提供的、携带有基质细胞衍生因子-1(stromal cell derived factor-1,SDF-1)cDNA的质粒pCMV-SPORT6中获取SDF-1的cDNA全长,并构建SDF-1-pIRES2-EGFP真核表达载体。方法采用双酶切、回收SDF-1cDNA片段,克隆至pIRES2-EGFP真核表达载体,得到SDF-1-pIRES2-EGFP真核表达载体。结果酶切及测序结果表明SDF-1-pIRES2-EGFP真核表达载体构建成功。结论获得SDF-1基因,构建SDF-1-pIRES2-EGFP真核表达载体,为探索SDF-1修饰人骨髓间充质干细胞(Mesenchymal stem cells,MSCs)促进人CD34+细胞归巢及增殖方面的作用奠定基础。

SDF-1通过活化PKC-ζ趋化人表皮干细胞定向迁移的实验研究

目的探讨信号蛋白PKC-ζ在间质细胞衍生因子1(stromal-derived factor 1,SDF-1)趋化人表皮干细胞定向迁移中的作用及机制。方法Ⅳ型胶原快速分选,无血清培养基(DK-SFM)培养表皮干细胞,免疫组化染色观察表皮干细胞β1整合素(β1 integrin)和角蛋白19(K19)的表达;Transwell实验观察SDF-1对钙和DAG依赖性和非依赖性PKC亚型抑制剂(chelerythrine chloride)、钙和DAG依赖性PKC亚型抑制剂(staurosporine)和PKC-ζ特异性抑制剂(PS-ζ)处理后人表皮干细胞的趋化作用;Western blot法检测SDF-1诱导后不同时段的人表皮干细胞PKC-ζ的磷酸化水平变化;采用Phal-loidin-Rhodamine显示细胞骨架,激光共聚焦显微镜观察PS-ζ对人表皮干细胞极化的影响。结果体外分离培养出人表皮干细胞,免疫组化染色显示,细胞质中β1整合素及K19均呈阳性表达。Transwell实验表明chelerythrine chloride和PS-ζ能够抑制SDF-1趋化的表皮干细胞运动,与阳性对照组比较差异有显著性(P<0.05)。SDF-1作用表皮干细胞能够引起PKC-ζ的磷酸化水平变化,随时间增加逐渐增强;激光共聚焦扫描显示SDF-1处理过的表皮干细胞骨架明显变化,经PS-ζ预处理后细胞骨架变化不明显。结论 SDF-1通过诱导信号蛋白PKC-ζ的磷酸化,影响细胞肌动蛋白的极化,趋化人表皮干细胞的定向迁移。

包载rhBMP-2和SDF-1的双层纳米微球的构建及体外释药研究

目的:构建搭载基质细胞衍生因子1(SDF-1)和人骨形态发生蛋白2(rh BMP-2)的双层纳米微球缓释系统,研究其体外释药特性。方法:用"乳化-溶剂挥发法"制备聚乳酸/壳聚糖(PLA/CS)双层纳米微球,通过正交试验获得最佳制备参数;动态光散射法测定纳米微球的粒径,电镜观察纳米微球的形态;在乳化过程中将rh BMP-2和SDF-1依次加入纳米微球中,计算其包封率和载药量,透析袋扩散法检测其体外缓释效果。结果:制备的双层纳米微球外形圆整,表面光滑,平均粒径为(542.33±14.38)nm,微球之间无粘连。rh BMP-2包封率为(82.41±1.05)%,载药量为(24.67±0.43)ng/mg;SDF-1包封率为(75.58±0.84)%,载药量为(22.63±0.41)ng/mg。药物释放持续至少30 d,呈"双相释放"。第30天时累计释放的rh BMP-2和SDF-1分别为72.85%和91.01%。结论:成功制备了包裹SDF-1和rh BMP-2的双层载药微球,形态良好,包封率较高,体外缓释效果较好。

雷珠单抗联合玻璃体切割术对PDR患者血清VEGF-A和SDF-1表达的影响

目的:探讨雷珠单抗联合玻璃体切割术(VT)对PDR患者血清VEGF-A、人基质细胞衍生因子1(SDF-1)表达的影响。方法:选取2017-01/2018-01本院收治的PDR患者120例,依据随机数字表法分为A组和B组,每组60例,A组给予VT治疗,B组在此基础上给予玻璃体腔注射雷珠单抗治疗,比较两组VT手术情况、并发症及VEGF-A、SDF-1、BCVA、CMT。结果:两组术后血清VEGF-A、SDF-1水平明显低于术前,且B组明显低于A组(P<0.05);B组VT手术时间、电凝止血、术中出血及并发症发生率明显低于A组(P<0.05);两组术后1d, 3mo BCVA、CMT明显低于术前,且B组明显低于A组(P<0.05)。结论:雷珠单抗联合VT可有效降低PDR患者血清VEGF-A、SDF-1水平,减少VT创伤及并发症,且可有效改善患者BCVA、CMT。

康柏西普联合玻璃体切割术对糖尿病性黄斑水肿患者房水VEGF、SDF-1的影响

目的:探讨康柏西普联合玻璃体切割术(VT)对糖尿病性黄斑水肿(DME)患者房水血管内皮生长因子(VEGF)、人基质细胞衍生因子1(SDF-1)的影响。方法:选取2015年3月至2018年3月南方医科大学附属小榄医院眼科收治的DME患者100例(100眼),依据随机数字表法分为VT组和西普组,每组50例,VT组给予VT治疗,西普组在此基础上给予康柏西普玻璃体腔注射治疗,比较两组房水VEGF、SDF-1及并发症、黄斑中心视网膜厚度(CMT)、最佳纠正视力(BCVA)。结果:VT组并发症发生率明显低于西普组,差异有统计学意义(P<0.05);VT组和西普组术后房水VEGF、SDF-1明显低于术前,且VT组明显低于西普组,差异有统计学意义(P<0.05);VT组和西普组术后1 d、1个月、3个月CMT、BCVA明显低于术前,且VT组明显低于西普组,差异有统计学意义(P<0.05)。结论:康柏西普联合VT可有效改善DME患者房水VEGF、SDF-1,有利于减少并发症,且可有效改善患者BCVA、CMT,值得临床作进一步推广。

Is 1, 25-dihydroxyvitamin D_3 an ideal substitute for dexamethasone for inducing osteogenic differentiation of human adipose tissue-derived stromal cells in vitro?

Background Human adipose tissue-derived stromal cells （hADSCs） can be induced to differentiate along an osteoblastic lineage under stimulation of dexamethasone （DEX）. Recent studies, however, have questioned the efficacy of glucocorticoids such as DEX in mediating the osteogenesis process of skeletal progenitor cells and processed lipoaspirate cells. Is it possible to find a substitute for DEX？ Therefore, this study was designed to investigate osteogenic capacity and regulating mechanisms for osteoblastic differentiation of hADSCs by comparing osteogenic media （OM） containing either 1, 25-dihydroxyvitamin D3 （VD） or DEX and determine if VD was an ideal substitute for DEX as an induction agent for the osteogenesis of hADSCs. Methods Osteogenic differentiation of hADSCs was induced by osteogenic medium （OM） containing either 10 nmol/L VD or 100 nmol/L DEX. Differentiation of hADSCs into osteoblastic lineage was identified by alkaline phosphatase （ALP） staining, von Kossa staining, and reverse transcription-polymerase chain reaction assays for mRNA expression of osteogenesis-related genes such as type Ⅰ collagen （COL Ⅰ）, bone sialoprotein （BSP）, osteocalcin （OC）, bone morphogenetic protein （BMP）-2, BMP-4, BMP-6, BMP-7, runt-related transcription factor 2/core binding factor α1 （Runx2/Cbfal）, osterix （Osx）, and LIM mineralization protein- 1 （LMP- 1）. Results von Kossa staining revealed that the differentiated cells induced by both VD and DEX were mineralized in vitro. They also expressed osteoblast-related markers, such as ALP, COL Ⅰ, BSP, and OC. Runx2/Cbfal, Osx, BMP-6, and LMP-1 were upregulated during VD and DEX-induced hADSC osteoblastic differentiation, but BMP-4, BMP-7 were not. BMP-2 was only expressed in VD-induced differentiated cells. Conclusions VD or DEX-induced hADSCs differentiate toward the osteoblastic lineage in vitro. Runx2/Cbfal, Osx, BMP-2, BMP-6, and LMP-1 are involved in regulating osteoblastic differentiation of hADSCs, but BMP-4, BMP-7 are not. VD, but not DEX, induces expression of BMP-2 during osteogenic induction of hADSCs. VD is an ideal substitute for DEX for osteogenic induction of hADSCs.

血管内皮生长因子、基质细胞衍生因子-1基因对人微血管内皮细胞增殖、迁移、凋亡的影响

目的探讨血管内皮生长因子(VEGF)、基质细胞衍生因子?1(SDF?1)基因对人微血管内皮细胞(HMEC?1)增殖、迁移、凋亡的影响。方法体外培养HMEC?1,以小干扰RNA(siRNA)介导低表达VEGF、SDF?1处理细胞,分组为Ⅰ组(空白对照组)、Ⅱ组(转染非特异性对照组)、Ⅲ组(转染si VEGF组)、Ⅳ组(转染si SDF?1组)。检测各组细胞增殖、迁移、凋亡的情况。West?ern Blot检测细胞中VEGF、SDF?1的表达情况,MTT和流式细胞分析检测HMEC?1增殖和凋亡能力的变化情况,划痕愈合实验检测HMEC?1迁移能力。结果转染了VEGF165?siRNA后,Ⅲ组VEGF165、SDF?1蛋白的表达强度(0.48±0.07)、(0.62±0.08)均明显弱于Ⅰ组(1.92±0.42)、(1.29±0.38)和Ⅱ组(1.87±0.35)、(1.32±0.47),差异有统计学意义(t=9.836,8.279,7.846,8.045,P<0.05);转染了SDF?1?siRNA后,Ⅳ组SDF?1蛋白的表达强度(0.37±0.05)均明显弱于Ⅰ组和Ⅱ组(t=7.381,7.984,P<0.05),差异有统计学意义,而VEGF165蛋白表达变化差异无统计学意义(P>0.05)。Ⅰ组与Ⅱ组比较,VEGF165、SDF?1蛋白表达水平差异无统计学意义(P>0.05)。经siRNA转染后,Ⅲ组、Ⅳ组细胞均出现增殖抑制率(42.37±1.25)%、(29.15±1.32)%和凋亡率(21.6±1.8)%、(16.8±1.6)%明显增高,与Ⅰ组、Ⅱ组增殖抑制率0.00%、(0.24±0.02)%和凋亡率(4.9±0.4)%、(5.2±0.5)%比较,差异有统计学意义(P<0.05)。但Ⅲ组和Ⅳ组之间比较,Ⅲ组细胞增殖抑制率和凋亡率增高更显著,差异有统计学意义(t=6.217,5.487,P<0.05)。Ⅰ组与Ⅱ组比较,细胞增殖抑制率和凋亡率均差异无统计学意义(P>0.05)。细胞迁移实验中,Ⅰ组、Ⅱ组、Ⅲ组、Ⅳ组迁移距离分别为(579.65±11.59)μm、(553.76±9.47)μm、(234.72±10.28)μm、(318.36±9.95)μm,Ⅲ组和Ⅳ组细胞明显少于Ⅰ组和Ⅱ组,差异有统计学意义(t=10.972,9.894,8.426,7.904,P<0.05),而Ⅰ组与Ⅱ组之间,差异无统计学意义(P>0.05),其中Ⅲ组和Ⅳ组之间比较,Ⅲ组细胞明显少于Ⅳ组,差异有统计学意义(t=5.907,P<0.05)。结论VEGF、SDF?1基因均参能促进HMEC?1的增殖和迁移能力,并抑制HMEC?1的凋亡水平,从而可能在糖尿病血管病变发生发展中发挥作用,且在此过程中VEGF对SDF?1表达具有调节机制。

基质细胞衍生因子-1对炎症和正常来源的人牙周膜干细胞成骨分化能力的影响

目的通过体外培养炎症来源的人牙周膜干细胞(iPDLSCs)和正常来源的人牙周膜干细胞(hPDLSCs),比较基质细胞衍生因子-1(SDF-1)对于两种来源细胞的成骨分化作用。方法采用组织块酶消化法原代培养iPDLSCs和hPDLSCs,经有限稀释法纯化,通过流式细胞仪对干细胞表面标记物检测鉴定后,对其进行成骨诱导;MTT法检测并比较SDF-1对两种来源的细胞增殖能力的影响;茜素红染色检测SDF-1作用于两种来源的细胞后钙化骨量的表达;碱性磷酸酶法比较SDF-1作用于两者的成骨分化能力;逆转录聚合酶链反应(RT-PCR)法检测SDF-1作用于两种牙周膜干细胞前后成骨相关基因表达水平的变化。结果两种来源的牙周膜细胞经纯化后均阳性表达干细胞标记物。hPDLSCs较iPDLSCs增殖能力高;两种细胞经SDF-1成骨诱导培养后,成骨相关基因的表达水平均较诱导前明显上调(P<0.05),SDF-1在50、200ng·mL^-1时分别对iPDLSCs和hPDLSCs细胞成骨分化作用最明显(P<0.05)。结论正常来源和炎症来源的人牙周膜干细胞均具有成骨分化能力,SDF-1可增强两种来源的牙周膜干细胞的成骨分化能力。

中国汉族人SDF1-β编码区新多态性位点初步研究

为调查中国汉族人HIV 1相关基因SDF 1β的多态性特点 ,选择 4 5例健康汉族人 ,对SDF 1β编码区的 4个外显子进行PCR扩增 ,然后分别测序。用DNAstar软件分析测序结果 ,在编码区共发现 1个基因多态性 (SNP)位点 :192位G→T ,使赖氨酸变为天冬酰胺 ,突变频率为 8 9% ;1例单碱基缺失 :10 0位T缺失 (10 0ΔT) ,引起 34位氨基酸移码突变 ,到 5 9位氨基酸翻译提前终止。两者均为首次发现 ,其对HIV

稳定表达基质细胞衍生因子1α的内皮细胞系构建及其与单核细胞的粘附作用

目的构建稳定表达基质细胞衍生因子1α的ECV304细胞系,研究基质细胞衍生因子1α在单核细胞/内皮细胞粘附中的作用。方法将大鼠基质细胞衍生因子1α基因聚合酶链反应产物及质粒载体pcDNA3.1用EcoRⅠ进行酶切,去磷酸化,置于连接反应体系中进行连接,将连接产物氯化钙法转化DH5α菌。氨苄青霉素筛选并扩增阳性菌落,经酶切鉴定插入方向正确后,再用G418筛选、逆转录聚合酶链反应检测基质细胞衍生因子1α浓度,建立稳定转染ECV304细胞系。在6孔板上种植转染基质细胞衍生因子1α基因的ECV304细胞,加THP-1细胞37℃孵育30min,磷酸缓冲液轻洗3遍,去除未粘附细胞,倒置显微镜下计数上、下、左、右、中5个视野,取其平均值得到每个视野粘附单核细胞数。结果经逆转录聚合酶链反应检测证实,稳定表达基质细胞衍生因子1α的ECV304细胞系构建成功,细胞计数表明,转染ECV304细胞系粘附THP-1细胞数是转染空质粒的十几倍,CXCR4单抗基质细胞衍生因子1α多抗均显著减少其粘附力(P<0.01)。结论内源性基质细胞衍生因子1α能促进ECV304细胞与单核细胞的粘附。

Growth and activation of PI-3K/PKB and Akt by stromal cell-derived factor 1a in endometrial carcinoma cells with expression of suppressor endoprotein PTEN

Background Mutation or deletion in the phosphatase and tensin homologue deleted on chromosome ten （PTEN） gene has been identified as an important cause of endometrial carcinoma; stromal cell derived factor-1α （SDF-1α） exerts growth-promoting effects on endometrial cancer cells through activation of the PI-3 kinase/Akt pathway and downstream effectors such as extracellular-responsive kinase （ERK）. In this study, a plasmid containing the PTEN gene was transfected into Ishikawa cells to investigate the difference in growth and signal transduction between Ishikawa-PTEN and Ishikawa cells after SDF-1α stimulation, and to study mechanisms of the involvement of PTEN protein in endometrial carcinoma development. Methods Ishikawa cells were transfected with a plasmid （pLXSN-PTEN） containing the PTEN gene and a plasmid （pLXSN-EGFP） with enhanced green fluorescent protein （EGFP）. Cells were then screened to obtain Ishikawa-PTEN cells and Ishikawa-neo cells that can both stably express PTEN protein and EGFP. Expression of PTEN protein, phosphorylation levels of AKT and ERK （pAKT and pERK） and growth differences in Ishikawa-PTEN, Ishikawa-neo and Ishikawa cells before and after SDF-1α stimulation were then determined by Western blots and MTT assays. Results Western blot analysis showed that Ishikawa cells produced PTEN after transfection with the PTEN gene. At 15 minutes after SDF-1α stimulation, the pAKT level of Ishikawa-PTEN cells was lower than that of Ishikawa-neo cells and Ishikawa cells. There was no significant difference in pERK levels among the three cell lines. The positive effect of SDF-1α on Ishikawa-PTEN cells growth was markedly less than the effect on Ishikawa-neo and Ishikawa cells. However, in the absence of SDF-1α stimulation （baseline）, the pAKT level in Ishikawa-PTEN cells was less than that in Ishikawa cells. There was a significant difference in growth between the Ishikawa-PTEN cells and the Ishikawa-neo cells. Conclusions PTEN gene transfection can regulate the level of pAKT but not pERK in Ishikawa-PTEN cells. PTEN protein may suppress the growth-promoting effect of SDF-1α on endometrial carcinoma by inhibiting the PI-3K/AKT signal transduction pathway.

卵巢癌血清SDF-1、肿瘤标志物变化及联合检测诊断卵巢癌价值分析

目的 探究血清基质细胞衍生因子-1(SDF-1)、肿瘤标志物[癌抗原125(CA125)、人附睾蛋白4(HE4)、糖类抗原199(CA199)]水平变化,并分析上述指标联合诊断卵巢癌的价值.方法 选取2021年3月-2023年7月在贵州金域医学检验中心经病理检查确诊的卵巢肿瘤患者102例,其中良性肿瘤62例,卵巢癌40例.比较两组患者的临床资料及SDF-1、CA125、HE4、CA199水平差异,采用Logistic回归分析筛选卵巢癌的危险因素,通过绘制ROC曲线分析相关指标单一及联合诊断卵巢癌的价值.依据病理分期将卵巢癌患者划分为Ⅰ-Ⅱ期和Ⅲ-Ⅳ期两个亚组,分析不同分期与SDF-1、CA125、HE4、CA199水平的关系.结果 卵巢癌组患者SDF-1、CA125、HE4、CA199水平均高于良性肿瘤组(P<0.05).SDF-1、CA125、HE4、CA199为卵巢癌发生的危险因素(P<0.05).当SDF-1、CA125、HE4、CA199分别为4372.76pg/mL、118.15U/mL、247.00pmol/L、67.37U/mL时,其诊断卵巢癌的AUC分别为0.814、0.794、0.824、0.805(P<0.05).SDF-1、CA125、HE4、CA199联合诊断卵巢癌的AUC为0.978,敏感度与特异度分别为95.12%和90.16%,联合诊断效能均较SDF-1、CA125、HE4、CA199单一指标更高(Z=3.514、3.562、3.850、4.190,P<0.05).卵巢癌Ⅲ-Ⅳ期患者SDF-1、CA125、HE4、CA199水平高于Ⅰ-Ⅱ期(P<0.05),且SDF-1、CA125、HE4、CA199分别与卵巢癌分期呈正相关(r=0.518、0.456、0.419、0.527,P<0.05).结论 卵巢癌患者其SDF-1、CA125、HE4、CA199等肿瘤标志物水平表达异常升高,联合检测有助于提高临床卵巢癌的诊断准确率.

Dedifferentiated human umbilical cord mesenchymal stem cell reprogramming of endogenous hSDF-1a expression participates in neural restoration in hypoxic-ischemic brain damagerats

The transplantation of human umbilical cord mesenchymal stem cells(hUC-MSCs)can promote hypoxic-ischemic brain damage(HIBD)nerve repair,but finding suitable seed cells to optimize transplantation and improve treatment efficiency is an urgent problem to be solved.In this study,we induced hUC-MSCs into dedifferentiated hUC-MSCs(De-hUC-MSCs),and the morphology,stem cell surface markers,proliferation and tri-directional differentiation ability of the De-hUC-MSCs and hUC-MSCs were detected.A whole-gene chip was utilized for genome cluster,gene ontology and KEGG pathway analyses of differentially expressed genes.De-hUC-MSCs were transplanted into HIBD rats,and behavioral experiments and immunofluorescence assays were used to assess the therapeutic effect.A lentivirus vector for human stromal cell-derived factor-1(hSDF-1a)was constructed,and the role of hSDF-1a in the neuroprotective effect and mechanism of De-hUC-MSCs was verified.De-hUC-MSCs displayed similar cell morphology,stem cell surface marker expression,cell proliferation and even three-dimensional differentiation ability as hUC-MSCs but exhibited greater treatment potential in vivo.The reprogramming mechanism of hSDF-1a participated in the dedifferentiation process.By successfully constructing a stable hSDF-1a cell line,we found that De-hUC-MSCs might participate in nerve repair through the hSDF-1a/CXCR4/PI3K/Akt pathway.De-hUC-MSCs reprogramming of endogenous hSDF-1a expression may mediate the hSDF-1a/CXCR4/PI3K/Akt pathway involved in nerve repair in HIBD rats.

Apelin and vascular endothelial growth factor are associated with mobilization of endothelial progenitor cells after acute myocardial infarction

This study was designed to determine the levels of early endothelial progenitor cells （EPCs）, apelin, vascu- lar endothelial growth factor （VEGF） and stromal cell-derived growth factor-1 （SDF-1） after acute myocardial infarction （AMI）, and to investigate the relationships between these cytokines and early EPCs. Early EPCs, de- fined as CD133＋, KDR＋, and CD34~ cells, were quantified by flow cytometry. The levels of early EPCs and those cytokines in AMI patients were significantly different from those with coronary artery disease or controls （P 〈 0.05）. Plasma apelin levels were inversely correlated with Gensini score and early EPCs （both P 〈 0.01）. Early EPCs, VEGF and SDF-1 showed different patterns of changes in AMI patients during the first 24 h. The trend in the change of early EPCs was proportionally correlated with that of VEGF （P 〈 0.05）. AMI patients exhibited in- creased early EPCs with remarkably decreased apelin levels and enhanced VEGF levels.