Effects of serum containing natural cerebrolysin on glucose-regulated protein 78 and CCAAT enhancer-binding protein homologous protein expression in neuronal PC12 cells following tunicamycin-induced endoplasmic reticulum stress

BACKGROUND： Glucose-regulated protein 78 （GRP78）, a marker of endoplasmic reticulum stress, can prolong cell survival. Alternatively, CCAAT enhancer-binding protein homologous protein （CHOP）, a transcription factor specific for endoplasmic reticulum stress, can cause cell cycle arrest and cell apoptosis. OBJECTIVE： To study the protective effects of serum containing natural cerebrolysin on endoplasmic reticulum stress in tunicamycin-induced neuronal PC12 cells, and analyze the influence on GRP78 and CHOP expressions. DESIGN, TIME AND SETTING： A parallel controlled study was performed at the Institute of Integrated Western and Traditional Chinese Medicine, Shenzhen Hospital, Southern Medical University, between March 2006 and August 2008. MATERIALS： Adult Sprague-Dawley rats were perfused with natural Cerebrolysin aqueous extract （0.185 g/kg/d） to produce serum containing natural Cerebrolysin. Physiological saline was used to produce blank serum. PC12 cell line was provided by Shanghai Institute of Cell Biology, Chinese Academy of Science. Tunicamycin was provided by Sigma （St. Louis, USA）, and natural Cerebrolysin, containing ginseng, rhizoma gastrodiae, and gingko leaf （1：2：2）, by Shengzhen Institute of Integrated Western and Traditional Chinese Medicine. METHODS： PC12 cells were treated with DMEM culture media containing 10% blank serum （normal control group）, tunicamycin （1 μg/mL; model group）, and 5%, 10%, and 15% serum containing natural cerebrolysin and tunicamycin （1 μ g/mL; low-, moderate-, and high-dose serum containing natural cerebrotysin groups）, for 2 hours. MAIN OUTCOME MEASURES： PC12 cells were treated with tunicamycin for 48 hours after which apoptosis was measured using the TUNEL method to calculate apoptotic index. GRP78 expression was detected using immunocytochemistry. After 24 hours of treatment with tunicamycin, GRP78 and CHOP mRNA expressions were measured using RT-PCR. RESULTS： The apoptotic index and CHOP mRNA expression were in the model group and three cerebrolysin groups were significantly increased when compared to the normal control group （P 〈 0.05）. In contrast, GRP78 mRNA and protein expressions were significantly decreased （P 〈 0.05）. CONCLUSION： Serum containing natural cerebrolysin significantly reduced apoptosis in neuronal PC12 cells following tunicamycin-induced endoplasmic reticulum stress. These results may be related to an up-regulation of GRP78 expression and down-regulation of CHOP expression, both of which displayed dose-dependent effects.

CCAAT/增强子结合蛋白α对K562细胞分化和凋亡的影响及其机制

目的:研究CCAAT/增强子结合蛋白α(CCAAT/enhancer-binding protein-alpha,C/EBPα)对K562细胞株分化和凋亡的影响及对相关基因的调控,为慢性粒细胞白血病的治疗提供新的治疗靶点。方法:将C/EBPα表达质粒pEGFP-C/EBPα及空载体对照质粒pEGFP分别经阳离子脂质体2000介导转染K562细胞,用G418筛选出C/EBPα稳定表达细胞株。Wright-Giemsa染色观察细胞形态学变化,FCM分析细胞表面分化抗原CD11b的表达、细胞周期及细胞凋亡,电子显微镜观察细胞凋亡,RT-PCR和Western印迹法检测细胞中相关基因Per2、cyclin B1和C-myc的表达。结果:筛选得到稳定表达C/EBPα的细胞株pEGFP-C/EBPα-K562。与空载体转染组及对照组细胞相比,转染组K562细胞分化明显,同时粒系细胞表面分化抗原CD11b表达增加;细胞周期分析发现,转染组细胞中G2期细胞增多,与空载体组和对照组相比,差异有统计学意义(P<0.05),同时出现细胞凋亡峰。细胞凋亡检测结果显示,转染组细胞凋亡明显增加(21.1%),与空载体组(6.0%)和对照组(4.2%)比较,差异有统计学意义(P<0.05);电子显微镜观察发现,转染组细胞中出现染色质浓集、断裂和核固缩等现象,并见凋亡小体;RT-PCR和Western印迹法检测发现,C/EBPα明显上调Per2 mRNA和蛋白表达,抑制cyclinB1、C-myc mRNA和蛋白的表达。结论:C/EBPα能促进K562细胞分化,并诱导细胞凋亡,其机制可能是通过对细胞周期相关基因的调控来实现的。

Notch1/Hes1信号调控CCAAT/增强子结合蛋白α表达对高氧损伤肺泡Ⅱ型上皮细胞增殖与分化的影响

背景:Notch1/Hes1信号和CCAAT/增强子结合蛋白α(CCAAT/enhancer-binding protein alpha,C/EBPα)在肺发育及肺损伤中均发挥重要作用。前期研究发现,高氧可引起肺泡Ⅱ型上皮细胞(typeⅡalveolar epithelialcell,AECII)增殖分化异常,并与C/EBPα异常表达有关,而这种异常是否与Notch1/Hes1信号调控有关,目前尚不清楚。目的:探讨Notch1/Hes1信号调控C/EBPα表达对高氧损伤AECII增殖与分化的影响。方法:体外培养人AECII,将细胞随机分为空气组、空气激活剂组(Notch通路激活剂Jagged1蛋白500μg/L)、高氧组(按3 L/min通入体积分数95%O_2和5%CO_2高纯混合气体且持续10 min)、高氧激活剂组(在通氧前30min加入Notch通路激活剂Jagged1蛋白500μg/L)。于干预后24h收获各组细胞,采用RT-PCR和Western blot法分别检测Notch1、Hes1及C/EBPαmRNA与蛋白表达水平;CCK-8法检测AECII细胞增殖;流式细胞术标记肺泡Ⅰ型上皮细胞特异性表面标志蛋白AQP5检测AECII分化。结果与结论:与空气组比,空气激活剂组Notch1、Hes1、C/EBPαmRNA和蛋白表达显著增加(P <0.05),AECII增殖增加而分化减少(P<0.05);高氧组和高氧激活剂组Notch1、Hes1、C/EBPαmRNA和蛋白表达显著降低(P <0.05),AECII增殖减少而分化增加(P <0.05);与高氧组比,高氧激活剂组Notch1、Hes1、C/EBPαmRNA和蛋白表达增加(P <0.05),AECII增殖增加而分化减少(P <0.05);结果提示,Notch1/Hes1信号可调控C/EBPα表达并能影响高氧损伤AECII增殖与分化功能。

Yinchenhao decoction attenuates obstructive jaundice-induced liver injury and hepatocyte apoptosis by suppressing protein kinase RNA-like endoplasmic reticulum kinase-induced pathway

BACKGROUND Chronic biliary obstruction results in ischemia and hypoxia of hepatocytes,and leads to apoptosis.Apoptosis is very important in regulating the homeostasis of the hepatobiliary system.Endoplasmic reticulum(ER)stress is one of the signaling pathways that induce apoptosis.Moreover,the protein kinase RNA-like endoplasmic reticulum kinase(PERK)-induced apoptotic pathway is the main way;but its role in liver injury remains unclear.Yinchenhao decoction(YCHD)is a traditional Chinese medicine formula that alleviates liver injury and apoptosis,yet its mechanism is unknown.We undertook this study to investigate the effects of YCHD on the expression of ER stress proteins and hepatocyte apoptosis in rats with obstructive jaundice(OJ).AIM To investigate whether YCHD can attenuate OJ-induced liver injury and hepatocyte apoptosis by inhibiting the PERK-CCAAT/enhancer-binding protein homologous protein(CHOP)-growth arrest and DNA damage-inducible protein 34(GADD34)pathway and B cell lymphoma/leukemia-2 related X protein(Bax)/B cell lymphoma/leukemia-2(Bcl-2)ratio.METHODS For in vivo experiments,30 rats were divided into three groups:control group,OJ model group,and YCHD-treated group.Blood was collected to detect the indicators of liver function,and liver tissues were used for histological analysis.For in vitro experiments,30 rats were divided into three groups:G1,G2,and G3.The rats in group G1 had their bile duct exposed without ligation,the rats in group G2 underwent total bile duct ligation,and the rats in group G3 were given a gavage of YCHD.According to the serum pharmacology,serum was extracted and centrifuged from the rat blood to cultivate the BRL-3A cells.Terminal deoxynucleotidyl transferase mediated dUTP nick end-labelling(TUNEL)assay was used to detect BRL-3A hepatocyte apoptosis.Alanine aminotransferase(ALT)and aspartate transaminase(AST)levels in the medium were detected.Western blot and quantitative real-time polymerase chain reaction(qRT-PCR)analyses were used to detect protein and gene expression levels of PERK,CHOP,GADD34,Bax,and Bcl-2 in the liver tissues and BRL-3A cells.RESULTS Biochemical assays and haematoxylin and eosin staining suggested severe liver function injury and liver tissue structure damage in the OJ model group.The TUNEL assay showed that massive BRL-3A rat hepatocyte apoptosis was induced by OJ.Elevated ALT and AST levels in the medium also demonstrated that hepatocytes could be destroyed by OJ.Western blot or qRT-PCR analyses showed that the protein and mRNA expression levels of PERK,CHOP,and GADD34 were significantly increased both in the rat liver tissue and BRL-3A rat hepatocytes by OJ.The Bax and Bcl-2 levels were increased,and the Bax/Bcl-2 ratio was also increased.When YCHD was used,the PERK,CHOP,GADD34,and Bax levels quickly decreased,while the Bcl-2 levels increased,and the Bax/Bcl-2 ratio decreased.CONCLUSION OJ-induced liver injury and hepatocyte apoptosis are associated with the activation of the PERK-CHOP-GADD34 pathway and increased Bax/Bcl-2 ratio.YCHD can attenuate these changes.

敲减CCAAT/增强子结合蛋白α通过增加O-GlcNAc糖基化水平促进肝癌细胞体外增殖

目的探讨CCAAT/增强子结合蛋白α(C/EBPα)在肝癌细胞增殖中的作用及其机制。方法利用靶向C/EBPα的RNAi慢病毒感染Hep3B肝癌细胞系,构建C/EBPα肝癌细胞系敲减模型。采用q RT-PCR和Western blot分别检测C/EBPαm RNA和蛋白表达水平,采用CCK-8检测敲减C/EBPα后对Hep3B细胞增殖的影响,采用在正常高葡萄糖(NG,4.5 g/L)和低葡萄糖(LG,1 g/L)条件下培养细胞的增殖变化,采用Western blot法检测不同葡萄糖浓度条件下在C/EBPα敲减细胞和对照细胞乙酰葡糖胺转移酶(OGT)、乙酰葡糖胺水解酶(OGA)和整个O-Glc NAc糖基化水平。结果靶向C/EBPα的RNAi慢病毒感染Hep3B肝癌细胞后,C/EBPαm RNA水平下调了(7.5±2.3)倍(P<0.05),蛋白表达水平下调了(8.8±0.25)倍(P<0.001),提示C/EBPα敲减细胞系构建成功;敲减C/EBPα后明显促进肝癌细胞的体外增殖;在低葡萄糖条件下刺激48 h和72 h,敲减C/EBPα分别促进细胞增殖15.4%(P<0.05)和25.0%(P<0.01);敲减C/EBPα后细胞OGA蛋白表达水平在正常高糖和低糖刺激24 h和48 h时分别下调了70.1%(P<0.01)、51.4%(P<0.05)和61.2%(P<0.05),整体O-Glc NAc糖基化表达水平上调,在低糖刺激48 h时升高80.6%。结论敲减转录因子C/EBPα可以提高细胞整体O-Glc NAc糖基化水平,从而促进肝癌细胞的体外增殖。

C/EBPα通过结合鸡神经调节蛋白4基因外显子2正调控其表达

神经调节蛋白4(NRG4)是一个新发现的脂肪细胞因子,它在机体能量平衡、糖脂代谢等许多生理过程中发挥重要调控作用。目前,NRG 4基因的转录调控机制尚不清楚。我们前期的5′RACE分析显示,鸡NRG 4基因转录起始位点(TSS)弥散分布于一段约200 bp的区域,提示鸡NRG 4基因的启动子为分散型启动子(dispersed promoter)。本研究开展了鸡NRG 4基因近端外显子和内含子的启动子活性分析,报告基因分析显示,包含NRG 4基因外显子1、内含子1和外显子2的基因组片段(-122/+452)具有很强的双向启动子活性。生物信息学分析显示,鸡NRG 4基因外显子2上存在1个转录因子CCAAT增强子结合蛋白α(C/EBPα)的潜在结合位点;报告基因分析发现,删除或突变C/EBPα结合位点会导致C/EBPα丧失对NRG 4基因片段(-122/+452)启动子活性的调控作用。基因表达相关性分析显示,鸡脂肪组织中C/EBPα和NRG 4基因的mRNA表达存在显著正相关(P<0.01)。进一步的脂肪组织ChIP-qPCR分析显示,C/EBPα直接结合鸡NRG 4基因的外显子2。本研究发现,鸡NRG 4基因的近端外显子和内含子具有双向启动子活性,C/EBPα通过直接结合外显子2调控鸡脂肪组织NRG 4基因的表达。

初治急性髓系白血病患者CEBPA基因突变检测及其临床意义

目的:探讨急性髓系白血病(AML)患者CCAAT/增强子结合蛋白-α(CEBPA)基因突变的情况,阐明其临床意义。方法:无菌采集279例AML患者和40名对照者骨髓或外周血样本,瑞士染色分析细胞形态学及骨髓幼稚细胞(BM Blast)比例;采用PCR联合序列分析法检测CEBPA、FLT3-ITD、NPM1和C-KIT基因突变情况;G显带技术进行染色体核型分析。结果:279例初治AML患者中35例检测到CEBPA基因突变,总检出率为12.5%,其在M2型患者中的检出率显著高于其他亚型(P<0.05)。35例突变患者中31例为双突变,其余4例为单突变,对照者CEBPA突变均为阴性。CEBPA基因突变常见于正常核型患者。与CEBPA野生型患者比较,CEBPA双突变患者的白细胞(WBC)计数、红细胞(RBC)计数及血红蛋白(HGB)水平升高(P<0.05),年龄、血小板(PLT)计数降低(P<0.05),而性别、BM blast比例及FLT3-ITD、NPM1、C-KIT基因突变发生率组间比较差异无统计学意义(P>0.05)。在治疗方面,CEBPA双突变型与野生型患者首疗程诱导缓解率分别为84.0%和80.5%(P>0.05)。结论:CEBPA基因突变主要见于M2亚型的AML患者,常见突变形式为双等位基因突变,CEBPA双突变型与野生型患者有不同临床特征,表现为WBC、RBC计数和HGB水平较高,年龄和PLT计数较低。

益髓生血颗粒对辐射损伤小鼠骨髓细胞C/EBPα、GM-CSF、GM-CSFRα、MAFB mRNA表达的影响

目的观察益髓生血颗粒对辐射损伤小鼠骨髓细胞CCAAT增强子结合蛋白α(C/EBPα)、粒-单系祖细胞集落刺激因子(GM-CSF)、粒-单系祖细胞集落刺激因子受体α(GM-CSFRα)、转录因子MAFB mRNA表达的影响,探讨该药调控骨髓造血的作用机制。方法采用随机数字表法将78只雄性昆明小鼠随机分为正常组、模型组、粒系祖细胞集落刺激因子(G-CSF)组及益髓生血颗粒高、中、低剂量组。益髓生血颗粒高、中、低剂量组先预防给药2 d,分别按12、6、3 g/(kg·d)灌胃。采用^(60)Co-γ射线全身一次性照射造模。造模第2天,G-CSF组按30μg/(kg·d)皮下注射G-CSF注射液,益髓生血颗粒高、中、低剂量组给药方法同预防给药,其余组均给予等量蒸馏水,连续14 d。进行小鼠骨髓细胞计数;采用实时荧光定量PCR(Q-PCR)检测骨髓细胞C/EBPα、GM-CSF、GM-CSFRα、MAFB mRNA表达。结果益髓生血颗粒能明显提高辐射损伤小鼠骨髓细胞计数(均P<0.05),上调骨髓细胞GM-CSF、GM-CSFRα、MAFB m RNA表达(均P<0.05),以低剂量组效果最佳。结论益髓生血颗粒可促进骨髓造血,其机制与上调骨髓细胞GM-CSF、GM-CSFRα、MAFB mRNA表达有关。

多聚胞嘧啶结合蛋白E2的RNA干扰对白血病32DP210细胞分化影响的分子机制探讨

目的:Bcr/abl诱导多聚胞嘧啶结合蛋白E2[poly(rC)-binding protein-E2,hnRNP-E2]的异常表达在慢性粒细胞白血病(chronic myeloid leukemia,CML)急变中起着重要作用。本研究旨在探讨hnRNP-E2特异性小发夹RNA(shor thairpin RNA,shRNA)对小鼠白血病32DP210细胞分化的影响,并初步探讨其可能的分子机制。方法:构建能表达特异性抑制小鼠hnRNP-E2基因表达的shRNA(即sh-hnRNP-E2)反转录病毒载体,经Phoenix-Ampho细胞包装后,取上清液感染小鼠白血病32DP210细胞,然后采用RT-PCR和Western印迹法验证sh-hnRNP-E2对hnRNP-E2 mRNA的干扰以及蛋白表达抑制效果,瑞氏染色法观察靶细胞分化情况,FCM法检测粒系分化抗原Gr-1表达情况,Western印迹法检测下游野生型CCAAT增强子结合蛋白α(CCAAT/enhancer-binding protein α,C/EBPα)的表达情况。结果:sh-hnRNP-E2反转录病毒感染32DP210细胞后,显著抑制靶细胞内hnRNP-E2 mRNA和蛋白的表达;靶细胞形态学出现粒系分化特征,细胞表面粒系分化抗原Gr-1表达被诱导;同时,靶细胞内野生型C/EBPα蛋白的表达恢复。结论:sh-hnRNP-E2特异性沉默靶细胞内hnRNP-E2基因表达后,可促进32DP210细胞向粒系分化;其机制可能与hnRNP-E2表达受抑制后,不能再对C/EBPα的翻译模式进行异常调控,从而恢复野生型C/EBPα的表达有关。

C/EBPα-Per2信号通路对K562细胞相关基因的调控机制

目的探索Per2在CCAAT增强子结合蛋白α(C/EBPα)参与调控的慢性粒细胞白血病(CML)发生、发展中的作用。方法通过脂质体介导将真核表达载体pGenesil-3-SiPer2和空载体pGenesil-3-HK转染到pEGFP-C/EBPα-K562细胞,利用新霉素筛选稳定干扰Per2的pEGFP-C/EBPα-K562单克隆细胞株。利用RT-PCR和Western blot分别检测转染组、空载组、对照组细胞p53、c-myc、cyclinB1的mRNA及蛋白表达水平的改变。结果成功构建稳定干扰Per2表达的pEGFP-C/EBPα-K562细胞株。与对照组和空载组细胞相比,转染组pGenesil-3-SiPer2-K562细胞的p53mRNA及蛋白表达水平明显降低,差异有统计学意义(P<0.01),而cyclinB1和c-myc基因的mRNA及蛋白表达水平则显著升高,差异有统计学意义(P<0.01)。结论 Per2基因在C/EBPα参与调控的CML发生发展中起重要作用,该通路的发现对于研究CML的发生及调控机制具有重要意义。

I血型系统研究进展

I血型系统包括1个抗原,I抗原。i抗原则归于集合207,而两者决定簇都存在于糖脂与糖蛋白所携带的碳水化合物结构上。i抗原是一种N-乙酰半乳糖胺重复单位,其是直链型的,其转化为I抗原的过程也就是该单位的支链化,而β-1,6-N-乙酰葡萄糖胺转移酶就必不可少了。在此基础之上,为了明确相关领域如成人i与先天性白内障的关系、出生后多聚-Lac NAc链直链向支链转变的分子机制等,以及确定I血型系统的研究进展关系着能否对相关血液学紊乱的病因、病理机制做进一步阐明,探索治疗及预防的最佳办法,我们需要展开更多的深入研究,系统回顾该领域的知识,搜索重要进展及新观点,综合分析有关实验结论与数据,从而为未来的研究指明方向。

1,25-二羟基维生素D_3抑制脂肪细胞分化作用的研究

目的研究1,25-二羟基维生素D3[1,25(OH)2D3]对脂肪细胞分化的影响及其机制。方法以间充质干细胞系C3H10T1/2为研究对象,将其分为6组,分别为对照组、诱导分化组和4个不同剂量的1,25(OH)2D3处理组。其中对照组加入溶媒,诱导分化组加入脂肪细胞诱导分化试剂,1,25(OH)2D3处理组除了加入脂肪细胞诱导分化试剂外,予以10-9、10-8、10-7、10-6mol/L 1,25(OH)2D3处理。处理后5 d进行油红O染色,RT-PCR检测脂肪细胞特异性转录因子和Wnt/β-catenin信号通路相关因子表达水平,Western blot检测β-catenin蛋白水平。结果1,25(OH)2D3能够强烈抑制脂肪细胞生成,阻断脂肪细胞特异性转录因子过氧化物酶体增殖物激活受体(PPAR)γ、CCAAT增强子结合蛋白(C/EBP)α及脂肪细胞表征因子aP2 mRNA表达,下调Wnt/β-catenin信号通路抑制因子分泌性卷曲相关蛋白1(sFRP1)mRNA,上调β连环素(β-catenin)蛋白水平。结论1,25(OH)2D3强烈抑制脂肪细胞分化,该作用可能与其激活Wnt/β-catenin信号通路有关。

转化生长因子B受体Ⅰ影响脂肪细胞分化的研究

目的探讨siRNA下调转化生长因子β受体Ⅰ(TGFBRⅠ)基因表达后对ST2细胞向脂肪细胞分化的作用。方法设计并合成针对TGFBRⅠ的靶向si RNA作为实验组,以转染Control si RNA作为对照组。应用q RT-PCR检测并比较转染ST2细胞后各组TGFBRⅠm RNA的表达和脂肪细胞特异性转录因子CCAAT增强子结合蛋白(C/EBP)α、过氧化物酶体增殖物激活受体(PPAR)γ、脂肪细胞表征因子FABP4 m RNA的表达水平。诱导5 d后对2组细胞进行油红O染色,检测TGFBRⅠsi RNA对ST2细胞分化的影响。利用激光共聚焦显微镜观察脂肪细胞的染色情况并对细胞进行拍照。另外,用异丙醇萃取出油红O,测定油红O在波长520 nm处的光密度(OD)值,并进行组间比较。结果转染TGFBRⅠsi RNA后,ST2细胞TGFBRⅠ基因的表达水平明显下调,TGFBRⅠsi RNA能够促进脂肪细胞生成,增强C/EBPα、PPARγ及FABP4 m RNA表达;经成脂诱导5 d后,转染TGFBRⅠsi RNA的细胞产生的脂滴明显较Control si RNA组多,且OD值高于Control si RNA组。结论 TGFBRⅠsi RNA能有效促进脂肪细胞的分化,提示TGFBRⅠ可能是前体细胞向脂肪细胞分化的重要调控因子。

L-4F Inhibits Oxidized Low-density Lipoprotein-induced Inflammatory Adipokine Secretion via Cyclic AMP/Protein Kinase A-CCAAT/Enhancer Binding Protein β Signaling Pathway in 3T3-L1 Adipocytes

Background： Adipocytes behave like a rich source of pro-inflammatory cytokines including monocyte chemoattractant protein- 1 （MCP- 1）. Oxidized low-density lipoprotein （oxLDL） participates in the local chronic inflammatory response, and high-density lipoprotein could counterbalance the proinftammatory function of αLDL, but the underlying mechanism is not completely understood. This study aimed to evaluate the effect of apolipoprotein A-I mimetic peptide L-4F on the secretion and expression of MCP-1 in fully differentiated 3T3-L 1 adipocytes induced by oxLDL and to elucidate the possible mechanisms. Methods： Fully differentiated 3T3-L 1 adipocytes were incubated in the medium containing various concentration of L-4F （0-50 gg/ml） with oxLDL （50 Lag/ml） stimulated, with/without protein kinase A （PKA） inhibitor H-89 （10 gmol/L） preincubated. The concentrations of MCP- 1 in the supematant, the mRNA expression of MCP- 1, the levels of CCAAT/enhancer binding protein α （C/EBPα）, and CCAAT/ enhancer binding protein 13 （C/EBPβ） were evaluated. The monocyte chemotaxis assay was performed by micropore filter method using a modified Boyden chamber. Results： OxLDL stimulation induced a significant increase ofMCP-1 expression and secretion in 3T3-L 1 adipocytes, which were inhibited by L-4F preincubation in a dose-dependent manner. PKA inhibitor H-89 markedly reduced the oxLDL-induced MCP-1 expression, but no further decrease was observed when H-89 was used in combination with L-4F （50 μg/ml） （P 〉 0.05）. OxLDL stimulation showed no significant effect on C/EBPa protein level but increased C/EBPβ protein level in a time-dependent manner. H-89 and L-4F both attenuated C/EBPI3 protein level in oxLDL-induced 3T3-L1 adipocytes. Conclusions： OxLDL induces C/EBPI3 protein synthesis in a time-dependent manner and enhances MCP-1 secretion and expression in 3T3-L 1 adipocytes. L-4F dose-dependently counterbalances the pro-inflammatory effect of oxLDL, and cyclic AMP/PKA-C/EBP-β signaling pathway may participate in it.

HNF1A、HNF1B、C/EBPA和ZHX2基因多态性与血清AFP水平相关性研究

目的探讨HNF1A-rs1169288(A/C)和rs2464196(G/A)、HNF1B-rs4430796(A/G)、C/EBPA-rs34529039(C/A)和ZHX2-rs7844465(G/T)基因多态性与中国健康成人血清甲胎蛋白(AFP)水平的相关性。方法纳入笔者医院2017年1~11月1010例年龄在25~65岁的汉族健康体检人员,采用等位基因特异性引物结合荧光定量PCR的方法(ARMS-TaqMan法)进行等位基因分型检测。血清AFP采用美国雅培公司i2000免疫分析仪测定。结果1010例研究对象的rs2464196最小等位基因A的频率为0.479。AFP水平在rs2464196-AA型(247例)最低,为3.60±1.59ng/ml,AG型(473例)为3.92±1.78ng/ml,GG型(290例)最高,为4.21±2.10ng/ml(P<0.001)。线性回归分析显示在控制影响AFP水平的各临床指标后,rs2464196基因多态性仍与血清AFP水平显著相关(P=0.000)。而HNF1A-rs1169288,HNF1B-rs4430796,C/EBPA-rs34529039和ZHX2-rs7844465多态性与血清AFP水平无显著相关。结论在表观健康成年人中,HNF1A-rs2464196A等位基因与血清AFP水平降低具有显著相关性,该发现为血清AFP水平变化提供了新的遗传决定因子。

CCAAT增强子结合蛋白α在甾醇类新药NSC67657诱导HL60细胞向单核系分化中的作用

目的探讨CCAAT增强子结合蛋白α（C／EBPα）在甾醇类新药NSC67657诱导HE60细胞向单核系分化中的作用。方法采用NSC67657诱导HL60细胞分化，流式细胞仪检测细胞表面分化抗原CD14的表达。应用逆转录聚合酶链反应（RT—PCR）和Western blot方法连续检测C／EBPα基因和蛋白在细胞分化前后的表达情况。构建pDsRed—C／EBPα真核表达载体，基因测序后采用电转染技术，将真核表达载体转入HL60细胞中，并进行表达验证。采用四甲基偶氮唑蓝（MTT）法、瑞氏染色和流式细胞技术，观察转染细胞在NSC67657作用前后的增殖和分化情况。结果10μmol／L NSC67657可以诱导HL60细胞向单核系分化，连续诱导5d后，有93．9％的细胞有CD14阳性表达。分化后的HL60细胞中，C／EBPα基因和蛋白表达均先升高后下降，分别在第2天和第3天达到峰值。真核表达载体构建成功，通过电转染和G418筛选，可获得90％以上阳性克隆。C／EBPα高表达可使HE60细胞增殖明显减缓，表面抗原CD11b的表达可达到（50．44±4．92）％。在NSC67657处理的重组质粒转染HL60细胞中，细胞单核系分化受到抑制，保留部分粒系分化。结论NSC67657诱导HL60细胞向单核系分化不一定通过C／EBPα蛋白的协调作用，但C／EBPα蛋白高表达可以阻止NSC67657诱导HL60细胞向单核系分化的进程。

人CCAAT增强子结合蛋白α基因影响骨肉瘤细胞生长活性研究

目的构建带Myc(p XJ-40)标签的CCAAT增强子结合蛋白α(CCAAT enhancer binding proteinα,C/EBPα)的真核表达载体,并检测其对骨肉瘤细胞生长的影响。方法应用聚合酶链式反应(polymerase chain reaction,PCR)技术从人乳腺文库中扩增出C/EBPα全长编码区基因;将扩增基因克隆到Myc载体中,并将重组质粒转染人胚胎肾293T细胞;Western blotting检测表达情况;另将重组Myc-C/EBPα质粒转染人骨肉瘤细胞系U2OS(实验组)、Myc空载体质粒转染U2OS细胞(对照组),生长实验检测C/EBPα对肿瘤细胞生长的影响。结果成功构建Myc-C/EBPα真核表达质粒,重组质粒转染人胚胎肾293T细胞后成功表达。生长实验显示Myc-C/EBPα转染的U2OS细胞的生长明显受限,随着培养时间延长,受抑制的程度逐渐增大,培养至第5天,Myc-C/EBPα转染的实验组细胞生长抑制率为58%,且细胞的生长速率OD=0.495明显低于空白对照组1.179,差异有统计学意义(P<0.01)。结论 C/EBPα对骨肉瘤细胞的生长具有抑制作用。

转录因子CCAAT／增强子结合蛋白α在银屑病皮损中的表达及意义

目的探讨转录因子CCAAT，增强子结合蛋白α（c／EBP—d）在寻常性银屑病皮损中的表达及与角质形成细胞异常增殖及皮损严重程度间的相关性。方法用免疫组化二步法及Westem印迹检测30例寻常性银屑病患者皮损和30例健康对照皮肤的表皮中C／EBP-α。免疫组化法检测Ki-67的表达，并根据Ki-67阳性表达数量计算增殖指数，Pearson相关分析法分析寻常性银屑病皮损中C／EBP-α的表达水平与角质形成细胞Ki一67增殖指数及银屑病皮损面积和严重程度指数（PASI评分）间的相关性。结果C／EBP—a主要在角质形成细胞胞质中表达，寻常性银屑病皮损中C／EBP—d的表达较健康对照皮肤明显下调（t=7．82，P〈0．05）。Ki-67主要在角质形成细胞胞核中表达，寻常性银屑病皮损中角质形成细胞的增殖指数明显高于健康对照皮肤（t=4．54，P〈0．05）。经Pearson相关分析，寻常性银屑病皮损中C／EBP-α表达水平与增殖指数呈负相关，与PASI评分呈负相关。Western印迹结果亦显示，C／EBP-α在银屑病皮损处的表达量显著下调。结论C／EBP—α在寻常性银屑病皮损中表达下调，可能参与了寻常性银屑病的发病过程。

雷公藤内酯通过CCAAT/增强子结合蛋白α抑制狼疮样肾炎小鼠IL-12/IL-23的表达

目的探究雷公藤内酯通过CCAAT/增强子结合蛋白α(CCAAT/enhancerbinding proteinα,C/EBPα)抑制狼疮样肾炎小鼠IL-12/IL-23表达的机制。方法实验分为3组:对照组(健康小鼠,n=15)、MRL/lpr组(狼疮样肾炎小鼠,n=15)和雷公藤内酯组(狼疮样肾炎小鼠经雷公藤内酯治疗,0.125 mg/kg/2 d,n=15);使用HITACHI-7080自动生化分析仪检测血清尿素氮和肌酸酐水平;用苏木素-伊红染色进行肾组织病理学测定,评估肾小球肾炎,间质性肾炎和血管病变的组织学评分;通过逆转录-实时定量PCR(RT-qPCR)和蛋白质印记分析了肾脏中炎性细胞因子(TNF-α、IL-6、IL-12和IL-23)mRNA和蛋白质表达;通过定点诱变将碱基取代检测IL-12/IL-23启动子活性;通过Ch IP测定小鼠C/EBP结合活性。结果与对照组(8.47±0.85,15.38±1.06)相比,MRL/lpr组尿素氮(29.14±2.05)和肌酸酐(40.18±3.72)水平增加(P<0.05),雷公藤内酯(11.36±1.23,20.17±2.45)治疗降低MRL/lpr小鼠尿素氮和肌酸酐水平(P<0.05);MRL/lpr组中的小鼠表现出肾损伤,组织学评分均增加(P<0.05),其特征在于系膜基质增加,管状铸型沉积和间质细胞浸润。相反,在雷公藤内酯处理的小鼠中这些病理特征改善;MRL/lpr组较对照组炎性细胞因子的mRNA和蛋白质表达增加(P<0.05)。雷公藤内酯降低了MRL/lpr小鼠中TNF-α、IL-6、IL-12和IL-23 mRNA和蛋白质表达(P<0.05);C/EBP的突变缓解雷公藤内酯对小鼠IL-12/IL-23启动子活性的抑制。结论雷公藤内酯通过C/EBPα抑制IL-12/IL-23的表达来改善MRL/lpr小鼠中的狼疮样肾炎。

DNA片段长度分析检测急性髓性白血病CEBPA基因突变

目的建立检测急性髓性白血病(AML)髓系转录因子CCAAT增强子结合蛋白-A(CEBPA)基因突变的快速筛查方法。方法采用聚合酶链式反应(PCR)扩增产物片段长度分析及序列分析方法检测107例初治AML患者CEBPA基因全部编码区突变情况。来自同种基因移植供者的38例正常人作为对照。结果同时用测序及片段长度分析的方法检测了107例AML患者及38例正常人CEBPA突变的情况,在排除了已知的多态位点以后,在107例AML患者中筛查出22例患者存在CEBPA突变,其中4例患者存在2种CEBPA突变,18例患者存在1种CEBPA突变,而在38例正常人中没有发现CEBPA突变。与测序结果比较,片段长度分析检测CEBPA突变是敏感和有效的。结论片段长度分析是一种快速、敏感地筛查CEBPA基因突变的方法,适合常规的AML诊断。