Resveratrol-downregulated Phosphorylated Liver Kinase B1 Is Involved in Senescence of Acute Myeloid Leukemia Stem Cells

Summary： Senescence is an important obstacle to cancer development. Engaging a senescent response may be an effective way to cure acute myeloid leukemia （AML）. The aim of this study was to examine the effect of resveratrol-downregulated phosphorylated liver kinase B1 （pLKB1） on the senescence of acute myeloid leukemia （AML） stem cells. The protein expressions of pLKB 1 and Sirtuin 1 （SIRT1）, a regulator ofpLKB1, were measured in CD34＋CD38-KGla cells treated with resveratrol （40 μmol/L） or not by Western blotting. Senescence-related factors were examined, including p21 mRNA tested by real-time PCR, cell morphology by senescence-associated β-galactosidase （SA-β-gal） staining, cell pro- liferation by MTT assay and cell cycle by flow cytometry. Besides, apoptosis was flow cytometrically determined. The results showed that pLKB1 was highly expressed in CD34＋CD38- KGla cells, and resveratrol, which could downregulate pLKB1 through activation of SIRT1, induced senescence and apoptosis of CD34＋CD38- KGla cells. It was concluded that resveratrol-downregulated pLKB1 is in- volved in the senescence of AML stem cells.

Interleukin-1 beta up-regulates tissue inhibitor of matrix metalloproteinase-1 mRNA and phosphorylation of c-jun N-terminal kinase and p38 in hepatic stellate cells

AIM： To study the relationship between interleukin-lbeta （IL-1β） up-regulating tissue inhibitor of matrix metalloproteinase-1 （TIMMP-1） mRNA expression and phosphorylation of both c-jun N-terminal kinase （INK） and p38 in rat heffatic stellate cells （HSC）. METHODS： RT-PCR was performed to measure the expression of TIMMP-1 mRNA in rat HSC. Western blot was performed to measure IL-1β-induced JNK and p38 activities in rat HSC. RESULTS： TIMMP-1 mRNA expression （1.191± 0.079） was much higher after treatment with IL-1β （10 ng/mL） for 24 h than in control group （0.545±0.091） （P〈0.01）. IL-1β activated INK and p38 in a time-dependent manner. After stimulation with IL-1β for 0, 5, 15, 30, 60 and 120 min, the INK activity was 0.982±0.299, 1.501±0.720, 2.133±0.882, 3.360±0.452, 2.181±0.789, and 1.385 ± 0.368, respectively. There was a significant difference in JNK activity at 15 min （P〈 0.01）, 30 min （P〈 0.01） and 60 min （P〈0.01） in comparison to that at 0 min. The p38 activity was 1.061±0.310, 2.050±0.863, 2.380±0.573, 2.973±0.953, 2.421±0.793, and 1.755 ± 0.433 at the 6 time points （0, 5, 15, 30, 60 and 120 min） respectively. There was a significant difference in p38 activity at 5 min （P〈0.05）, 15 min （P〈0.01）, 30 min （P〈0.01） and 60 min （P〈0.01） compared to that at 0 min. TIMMP-1 mRNA expression trended to decrease in 3 groups pretreated with different concentrations of SP600125 （10 μmol/L, 1.022±0.113; 20 μmol/L, 0.869±0.070; 40 μmol/L, 0.666±0.123）. Their decreases were all significant （P〈0.05, P〈0.01, P〈0.01） in comparison to control group （without SP600125 treatment, 1.163±0.107）. In the other 3 groups pretreated with different concentrations of SB203580 （10 μmol/L, 1.507±0.099; 20 μmol/L, 1.698±0.107; 40 μmol/L, 1.857±0.054）, the expression of TIMMP-1 mRNA increased. Their levels were higher than those in the control group （without SB203580 treatment, 1.027 ± 0.061） with a significant statistical significance （P〈 0.01）. CONCLUSION： IL-1β has a direct action on hepatic fibrosis by up-regulating TIMMP-1 mRNA expression in ratessionin in rate HSC.JNK and p38 mitogen-activated protein kinases （MAPKs） are involved in IL-1β-induced TIMMP-1 gene expression, and play a distinct role in this process, indicating that p38 and .INK pathways cooperatively mediate TIMP-1 mRNA expression in rat HSC.

Sphingosine kinase 1 dependent protein kinase C-δ activation plays an important role in acute liver failure in mice

AIM: To investigate the role of protein kinase C(PKC)-δ activation in the pathogenesis of acute liver failure(ALF) in a well-characterized mouse model of D-galactosamine(D-Gal N)/lipopolysaccharide(LPS)-induced ALF.METHODS: BALB/c mice were randomly assigned to five groups, and ALF was induced in mice by intraperitoneal injection of D-Ga IN(600 mg/kg) and LPS(10 μg/kg). Kaplan-Meier method was used for survival analysis. Serum alanine aminotransferase(ALT) and aspartate aminotransferase(AST) levels at different time points within one week were determined using a multiparameteric analyzer. Serum levels of high-mobility group box 1(HMGB1), tumor necrosis factor(TNF)-α, interleukin(IL)-1β, IL-6, and IL-10 as well as nuclear factor(NF)-κB activity were determined by enzyme-linked immunosorbent assay. Hepatic morphological changes at 36 h after ALF induction were assessed by hematoxylin and eosin staining. Expression of PKC-δ in liver tissue and peripheral blood mononuclear cells(PBMCs) was analyzed by Western blot.RESULTS: The expression and activation of PKC-δ were up-regulated in liver tissue and PBMCs of mice with D-Gal N/LPS-induced ALF. Inhibition of PKC-δ activation with rottlerin significantly increased the survival rates and decreased serum ALT/AST levels at 6, 12 and 24 h compared with the control group(P < 0.001). Rottlerin treatment also significantly decreased serum levels of HMGB1 at 6, 12, and 24 h, TNF-α, IL-6 and IL-1 β at 12 h compared with the control group(P < 0.01). The inflammatory cell infiltration and necrosis in liver tissue were also decreased in the rottlerin treatment group. Furthermore, sphingosine kinase 1(Sph K1) dependent PKC-δ activation played an important role in promoting NF-κB activation and inflammatory cytokine production in ALF.CONCLUSION: Sph K1 dependent PKC-δ activation plays an important role in promoting NF-κB activation and inflammatory response in ALF, and inhibition of PKC-δ activation might be a potential therapeutic strategy for this disease.

Serum levels of angiotensin converting enzyme as a biomarker of liver fibrosis

The renin angiotensin system(RAS) is classically conceived as a circulating hormonal system involved in blood pressure control and hydroelectrolyte balance. The discovery that RAS components are locally expressed in a wide range of organs and tissues,including the liver,pointed to a role for this system in the pathogenesis of several conditions including hepatic fibrosis and cirrhosis. It has been widely reported that the classical RAS axis composed by the angiotensin converting enzyme(ACE)-angiotensin(Ang) Ⅱ-Ang type 1(AT1) receptor mediates pro-inflammatory,pro-thrombotic,and pro-fibrotic processes. On the other hand,the alternative axis comprising ACE2-Ang-(1-7)-Mas receptor seems to play a protective role by frequently opposing Ang Ⅱ action. Chronic hepatitis B(CHB) is one of the leading causes of liver fibrosis,accounting for the death of nearly one million people worldwide. Liver fibrosis is a key factor to determine therapeutic interventions for patients with CHB. However,the establishment of non-invasive and accurate methods to detect reversible stages of liver fibrosis is still a challenge. In an elegant study published in the 36 th issue of the World Journal of Gastroenterology,Noguchi et al showed the predictive value of serum ACE levels in detecting not only advanced stages of liver fibrosis but also initial and intermediate fibrotic stages. The serum levels of ACE might represent an accurate,non-invasive,widely available,and easy method to evaluate fibrosis related to CHB. Moreover,therapies involving the inhibition of the classical RAS axis components might be promising in the control of CHB-related liver fibrosis.

用cDNA微阵列技术研究HBV X基因与AFB_1对HBVx转基因小鼠药物代谢酶基因表达谱的影响

目的 研究乙型肝炎病毒X基因和黄曲霉毒素诱发小鼠肝癌过程中药物代谢酶基因表达谱的变化,探讨两因素协同致肝癌的机制。方法 用BiostarM 40s微阵列芯片比较研究HBVx组、AFB1 组和(AFB1+HBVx)组的肝组织基因表达谱与对照组的差异。结果 各实验组分别与对照组相比基因表达谱发生了明显的改变,各实验组上调与下调的基因数目分别为(AFB1+HBVx)组69项;AFB1 组101项;HBVx组35 项;其中与代谢酶相关的基因有18 项表达发生改变,分别为(AFB1 +HBVx)组13项(13/18,72%);HBVx组4项(4/18,22%);AFB1 组8项(8/18,44%)。结论 小鼠受到HBV X基因和AFB1双重攻击后,其体内的GST、EPHX和UDPGT等药物代谢酶基因表达水平明显低于HBVx组和AFB1 组。HBV与AFB1 协同致癌的分子机制很可能与两者引起药物代谢酶基因表达水平下调有关。

LKB1在肝细胞癌中的表达及其对预后的影响

目的探讨LKB1基因在肝细胞性肝癌(HCC)中的表达及其与肝细胞癌患者预后的关系。方法采用免疫组化技术检测70例HCC患者肝癌及癌旁组织和20例正常肝组织中LKB1蛋白的表达,采用x2检验分析LKB1表达与临床病理因素的关系。对该组70例患者进行随访,并应用COX比例风险回归模型对其预后影响因素进行评估。结果 LKB1蛋白在HCC组织中的阳性表达率明显低于正常肝组织和癌旁组织(P<0.05)。HCC患者中,LKB1蛋白表达与HCC的分化程度,门静脉侵袭,TNM分期有关(P<0.05)。LKB1阳性表达的患者生存时间比阴性表达的显著延长(P<0.05)。门静脉侵袭、胆管癌栓、TNM分期和LKB1表达是影响HCC预后的独立危险因素(P<0.05)。结论 LKB1蛋白表达是影响HCC患者生存时间的独立因素之一,检测LKB1蛋白可能为HCC患者预后判断提供参考。

大黄酸通过Sirt1/AMPK信号通路对非酒精性脂肪性肝病小鼠肝功能及肝细胞脂代谢的影响

目的:研究不同浓度大黄酸灌胃通过沉默信息调节因子2相关酶1(Sirt1)/amp活化蛋白激酶(AMPK)信号通路对非酒精性脂肪性肝病(NAFLD)小鼠的肝功能及肝细胞脂代谢的影响。方法:实验小鼠分为空白组,模型组,低、高剂量大黄酸组和高剂量大黄酸+Sirt1抑制剂(高剂量大黄酸+EX527)组。动物实验:除空白组外其余各组小鼠采用连续饲喂高脂饲料(8周)构建NAFLD小鼠模型。8周干预完成后各组小鼠于处死前称重并记录,全自动生化分析仪检测血清总胆固醇(TC)、甘油三酯(TG)、丙二醛(MDA)、游离脂肪酸(NEFA)水平;ELISA法检测血清丙氨酸氨基转移酶(ALT)、天门冬氨酸氨基转移酶(AST)和肝脏组织乙酰辅酶羧化酶(ACC)水平;苏木精伊红染色(HE)及油红O染色检验肝组织硬化程度及细胞脂肪病变水平。细胞实验:采用200μmol/L棕榈酸(PA)处理AML-12细胞24 h构建NAFLD细胞模型。全自动生化分析仪检测TG含量;油红O染色观察AML-12细胞脂质积累情况;Western Blot法检测肝脏组织和AML-12细胞中Sirt1、AMPKα、磷酸化AMPKα(p-AMPKα)蛋白表达。结果:与空白组相比,模型组小鼠体重和肝脏湿重升高,肝脏组织明显损伤,AML-12细胞中TG含量及小鼠血清TG、TC、MDA、ALT、AST、NEFA水平显著升高,肝脏组织ACC含量降低(P<0.05),肝脏组织和AML-12细胞中Sirt1、p-AMPKα/AMPKα表达降低,脂肪病变严重,脂质积累增高(P<0.05)。与模型组相比,低、高剂量大黄酸组小鼠体重和肝脏湿重降低,肝脏组织损伤减轻,AML-12细胞中TG含量及小鼠血清TG、TC、MDA、ALT、AST、NEFA水平显著降低,肝脏组织ACC含量升高(P<0.05),肝脏组织和AML-12细胞中Sirt1、p-AMPKα/AMPKα表达升高,脂肪病变减轻,脂质积累降低(P<0.05)。与高剂量大黄酸组相比,高剂量大黄酸+EX527组各项指标均有所逆转(P<0.05)。结论:大黄酸可有效通过调节小鼠肝细胞脂代谢改善NAFLD小鼠肝功能水平,其机制可能与激活Sirt1/AMPK信号通路有关。

多囊卵巢综合征伴胰岛素抵抗相关信号通路的研究进展

多囊卵巢综合征(PCOS)是一种好发于青春期及育龄期女性的涉及诸多因素的内分泌代谢性疾病,临床主要表现为闭经、体胖、多毛痤疮以及妊娠率显著降低,但目前其病因病机尚不清楚。胰岛素抵抗(IR)与多种慢性非传染性疾病(高血压、糖尿病、心脑血管疾病、PCOS等)相关,目前已知磷脂酰肌醇-3-激酶/蛋白激酶B、肝激酶B1/AMP活化的蛋白激酶、沉默信息调节因子1/叉头框转录因子O1、Toll样因子4/核因子κB信号通路参与了PCOS伴IR(PCOS-IR)的作用机制,因此充分认识PCOS-IR的发病机制在疾病预防中有重要临床意义。

血清VEGF、TK-1和T淋巴细胞亚群与乙型肝炎病毒相关性肝病发生和进展的关系

目的:探讨血清血管内皮细胞生长因子(VEGF)、可溶性胸苷激酶-1(TK-1)和T淋巴细胞亚群与乙型肝炎病毒(HBV)相关性肝病的发生和进展的关系。方法:选择HBV相关性肝病病人188例,其中单纯乙型肝炎(乙肝)52例,肝纤维化40例,肝硬化56例,肝癌40例。另选择30名健康体检者为对照组。采用PCR法检测HBV-DNA负荷量,常规生化法检测肝功能指标丙氨酸氨基转移酶(ALT)和天冬氨酸氨基转移酶(AST)水平,ELISA法检测VEGF和TK-1水平,流式细胞术检测T淋巴细胞亚群CD3^(+)、CD4^(+)、CD8^(+)百分比和CD4^(+)/CD8^(+)。结果:单纯乙肝组、肝纤维化组、肝硬化组、肝癌组的HBV-DNA负荷量及ALT、AST水平差异均无统计学意义(P>0.05)。肝癌组、肝硬化组、肝纤维化组、单纯乙肝组、对照组VEGF和TK-1、CD4^(+)/CD8^(+)水平逐渐降低;各组CD3^(+)、CD4^(+)和CD8^(+)水平差异均无统计学意义(P>0.05)。HBV相关性肝病病人血清中VEGF与TK-1呈明显正相关关系(r=0.745,P<0.01),VEGF与CD4^(+)/CD8^(+)呈明显负相关关系(r=-0.217,P<0.01),TK-1与CD4^(+)/CD8^(+)呈明显负相关关系(r=-0.208,P<0.01)。结论:HBV相关性肝病病人血清中VEGF、TK-1和CD4^(+)/CD8^(+)水平与疾病的发生和进展相关,VEGF和TK-1表达升高、CD4^(+)/CD8^(+)下降可能参与了乙肝、肝纤维化、肝硬化和肝癌的发生和进展。

RIPK3基因转染的SH-SY5Y细胞中HIF-1α基因及其信号通路相关基因表达变化

目的观察受体相互作用蛋白激酶3(RIPK3)基因转染的神经母细胞瘤细胞系SH-SY5Y中低氧诱导因子1α(HIF-1α)mRNA及其信号通路相关基因表达变化。方法构建表达RIPK3基因的p CMV6-AC-GFP质粒(重组质粒),培养SH-SY5Y细胞,分为实验组及对照组,分别转染重组质粒和空载质粒。采用Western blotting法检测细胞中的RIPK3蛋白,分别于培养8、14、20、26、32、38 h后,通过MTT实验检测细胞增殖情况(OD值)。采用转录组测序技术(RNAseq)及Ingenuity Pathway Analysis(IPA)软件检测并筛选RIPK3-HIF1α下游信号通路中的关键基因。采用微滴式数字PCR(dd PCR)检测两组细胞中的HIF-1αmRNA。结果实验组细胞中RIPK3蛋白相对表达量(0.806±0.097 5)高于对照组(0.455±0.088 6),P<0.05。随培养时间延长,实验组细胞增殖受到抑制。实验组细胞中HIF-1αmRNA相对表达量(0.015 43±0.003 47)低于对照组(0.046 28±0.010 26),P<0.05。在HIF-1α为核心的相互作用关系网络中,筛选出关键分子泛素缀合酶样蛋白(UBC)、希佩尔-林道蛋白(VHL)、转录延伸因子B多肽1(TCEB1)、血管内皮生长因子A(VEGFA)。结论 RIPK3基因转染SH-SY5Y后,细胞中HIF-1αmRNA表达下调,同时HIF-1α信号通路相关基因(UBC、VHL、TCEB1、VEGFA)的表达水平受到影响。

LKB1 in lung cancerigenesis:a serine/threonine kinase as tumor suppressor

Lung cancer is featured with high mortality,with a 15%five-year survival rate worldwide.Genetic alterations,such as loss of function of tumor suppressor genes,frequently contribute to lung cancer initiation,progression and metastasis.Liver kinase B1(LKB1),as a serine/threonine kinase and tumor suppressor,is frequently mutated and inactivated in non-small cell lung cancer(NSCLC).Recent studies have provided strong evidences that LKB1 loss promotes lung cancerigenesis process,especially lung cancer progression and metastasis.This review will summarize recent progress on how LKB1 modulates the process of lung cancerigenesis,emphasizing on LKB1 downstream signaling pathways and biological functions.We will further discuss the potential development of prognostic biomarkers or therapeutic targets in lung cancer clinic based on the molecular alteration associated with deregulated LKB1 signaling.

Effect of cis-9,trans-11-conjugated linoleic acid on cell cycle of gastric adenocarcinoma cell line(SGC-7901)

AIM: To determine the effect of cis -9, trans -11-conjugated linoleic acid (c9, t11-CLA) on the cell cycle of gastric cancer cells (SGC-7901) and its possible mechanism in inhibition cancer growth. METHODS: Using cell culture and immunocytochemical techniques, we examined the cell growth, DNA synthesis, expression of PCNA, cyclin A, B(1), D(1), p16(ink4a) and p21(cip/waf1) of SGC-7901 cells which were treated with various c9, t11-CLA concentrations (25, 50, 100 and 200 micromol.L(-1))of c 9, t 11-CLA for 24 and 48h, with a negative control (0.1% ethane). RESULTS: The cell growth and DNA synthesis of SGC-7901 cells were inhibited by c9, t11-CLA.SGC-7901 cells. Eight day after treatment with various concentrations of c9, t11-CLA mentioned above, the inhibition rates were 5.92%, 20.15%, 75.61% and 82.44%, respectively and inhibitory effect of c9, t11-CLA on DNA synthesis (except for 25 micromol.L, 24h) showed significantly less (3)H-TdR incorporation than that in the negative controls (P【0.05 and P【0.01). Immunocytochemical staining demonstrated that SGC-7901 cells preincubated in media supplemented with different c9, t11-CLA concentrations at various times significantly decreased the expressions of PCNA (the expression rates were 7.2-3.0%, 24h and 9.1-0.9% at 48h, respectively), Cyclin A (11.0-2.3%, 24h and 8.5-0.5%,48h), B(1) (4.8-1.8% at 24h and 5.5-0.6% at 48h)and D(1) (3.6-1.4% at 24h and 3.7%-0 at 48h) as compared with those in the negative controls(the expressions of PCNA, Cyclin A, B(1) and D(1) were 6.5% at 24h and 9.0% at 48h, 4.2% at 24h and 5.1% at 48h, 9.5% at 24h and 6.0% at 48h,respectively)(P【0.01), whereas the expressions of P16(ink4a) and P21(cip/waf1), cyclin-dependent kinases inhibitors(CDKI), were increased. CONCLUSION: The cell growth and proliferation of SGC-7901 cell is inhibited by c9, t11-CLA via blocking the cell cycle, with reduced expressions of cyclin A,B(1) and D(1) and enhanced expressions of CDKI(P16(ink4a) and p21(cip/waf1)).

基质金属蛋白酶抑制剂-1在肝纤维化诊断中的临床应用

目的:评估血清基质金属蛋白酶抑制剂-1(TIMP-1)在肝纤维化诊断中的临床价值。方法:285例慢性乙型肝炎(CHB)患者,根据肝穿刺病理诊断结果分为无明显纤维化组(S0～S1)和明显纤维化组(S2～S4)。将病理诊断结果作为金标准,使用ROC曲线评估TIMP-1诊断肝纤维化的敏感度、特异性和符合率,并和肝纤维化标记物HA、PCⅢ、CⅣ、LN比较其诊断性能。结果:对照组、S0～S1组、S2～S4组TIMP-1血清浓度分别为(146.6±29.2)、(161.2±43.2)、(221.6±93.8)μg/L,对照组和S2～S4组及S0～S1组和S2～S4组间比较差异均有统计学意义(t分别为5.32、4.98,P<0.01)。TIMP-1区分慢性乙肝明显纤维化和轻度纤维化的ROC曲线下面积(AUC)为0.801(95%CI:0.762～0.940),TIMP-1在临界值为170.3μg/L时,其敏感度、特异度分别为88.5%、80.4%,高于HA(79.6%、72.5%),PCⅢ(72.5%、78.5%),CⅣ(63.6%、78.4%)和LN(78.5%、64.7%)。结论:血清TIMP-1诊断肝纤维化有较高的敏感度和特异性,血清TIMP-1可能是预测肝纤维化分期一个较好的指标。

APOBEC3B调控葡萄膜黑色素瘤复制应激的研究

目的·研究载脂蛋白B mRNA编辑酶催化亚基3B(apolipoprotein B mRNA editing enzyme catalytic subunit 3B,APOBEC3B)在葡萄膜黑色素瘤(uveal melanoma,UM)中的生物学功能以及对药物治疗敏感性的影响。方法·应用免疫组织化学染色和Western blotting,分别检测眼部黑色素瘤[UM和结膜黑色素瘤(conjunctival melanoma,CM)]组织和细胞中APOBEC3B蛋白的表达水平。通过检索癌症基因组图谱(The Cancer Genome Atlas,TCGA)数据库,分析UM中APOBEC3B表达水平与预后的关联。使用CRISPR-Cas9质粒APOBEC3B-sgRNA敲除UM细胞系OMM2.3中APOBEC3B基因,构建APOBEC3B敲除的OMM2.3稳转细胞系sgAPOBEC3B以及对照细胞系Vector;并通过克隆形成实验,探索APOBEC3B敲除对OMM2.3细胞增殖的影响。同时,通过APOBEC3B-shRNA和空载质粒建立APOBEC3B敲低的OMM2.3细胞shAPOBEC3B和对照细胞shCtrl,对其进行转录组测序(RNA sequencing,RNA-seq),检测差异基因,并通过基因集富集分析(gene set enrichment analysis,GSEA)揭示APOBEC3B调控的下游通路。通过免疫荧光染色鉴定下游通路的关键蛋白。通过应用通路靶向药物处理,检测APOBEC3B对UM药物治疗敏感性的影响。结果·免疫组织化学染色结果表明眼部黑色素瘤(UM和CM)组织相较于良性色素痣组织APOBEC3B表达更高。Western blotting也表明包括OMM2.3细胞在内的大多数眼部黑色素瘤细胞相较于正常对照细胞(视网膜色素上皮细胞)APOBEC3B蛋白表达水平更高。并且TCGA数据库分析表明,APOBEC3B高表达的UM患者总生存期(P=0.032)和无病生存期(P=0.000)更短。然而APOBEC3B敲除并不影响OMM2.3细胞克隆形成的能力,APOBEC3B敲低也没有造成细胞周期的显著改变。shAPOBEC3B和shCtrl细胞系的RNA-seq差异基因富集分析结果显示,APOBEC3B参与调控OMM2.3细胞的复制应激相关通路,并且热图分析也显示APOBEC3B敲低后DNA复制应激相关通路基因表达发生改变。免疫荧光染色结果显示,APOBEC3B敲低后复制应激通路关键靶标磷酸化的复制蛋白A 32 kDa亚基(replication protein A 32 kDa subunit,RPA32)水平降低。在对APOBEC3B敲低的OMM2.3细胞和对照细胞的药物敏感性实验中,发现相较于shAPOBEC3B细胞,shCtrl细胞对细胞周期检测点激酶1(cell cycle checkpoint kinase 1,CHK1)抑制剂的敏感性更高。结论·APOBEC3B参与调控OMM2.3细胞复制应激相关通路,且APOBEC3B表达的OMM2.3细胞对CHK1抑制剂的处理更为敏感。

C4.4A as a biomarker in pulmonary adenocarcinoma and squamous cell carcinoma

The high prevalence and mortality of lung cancer, together with a poor 5-year survival of only approximately 15%, emphasize the need for prognostic and predictive factors to improve patient treatment. C4.4A, a member of the Ly6/uP AR family of membrane proteins, qualifies as such a potential informative biomarker in non-small cell lung cancer. Under normal physiological conditions, it is primarily expressed in suprabasal layers of stratified squamous epithelia. Consequently, it is absent from healthy bronchial and alveolar tissue, but nevertheless appears at early stages in the progression to invasivecarcinomas of the lung, i.e., in bronchial hyperplasia/metaplasia and atypical adenomatous hyperplasia. In the stages leading to pulmonary squamous cell carcinoma, expression is sustained in dysplasia, carcinoma in situ and invasive carcinomas, and this pertains to the normal presence of C4.4A in squamous epithelium. In pulmonary adenocarcinomas, a fraction of cases is positive for C4.4A, which is surprising, given the origin of these carcinomas from mucin-producing and not squamous epithelium. Interestingly, this correlates with a highly compromised patient survival and a predominant solid tumor growth pattern. Circumstantial evidence suggests an inverse relationship between C4.4A and the tumor suppressor LKB1. This might provide a link to the prognostic impact of C4.4A in patients with adenocarcinomas of the lung and could potentially be exploited for predicting the efficacy of treatment targeting components of the LKB1 pathway.

蛋白激酶B1去类泛素化修饰抑制肝癌的增殖和转移

目的 探讨沉默泛素载体蛋白9（Ubc9）基因表达诱导蛋白激酶B1（AKT1）去类泛素化修饰,及其对肝癌细胞增殖和转移的影响.方法 利用RNA干扰技术沉默HepG2肝癌细胞Ubc9基因表达,Western blot法检测Ubc9、小泛素相关修饰蛋白1（SUMO1）和蛋白激酶B1（AKT1）蛋白表达水平,四甲基偶氮唑蓝（MTT）法和流式细胞术检测HepG2细胞增殖活性,细胞划痕实验和Transwell方法检测细胞迁移能力.建立荷瘤鼠模型,测量肿瘤体积并绘制生长曲线,解剖肿瘤组织并称重比较.采用原位细胞凋亡实验检测肿瘤组织细胞凋亡情况,免疫组化法检测肿瘤组织中增殖细胞核抗原（PCNA）、基质金属蛋白酶2（MMP-2）和 MMP-9的表达情况.结果 siR-Ubc9基因转染可使HepG2细胞中Ubc9、共轭SUMO1、游离SUMO1和AKT1蛋白水平均明显下降（均P〈0.05）.对照组、siR-neg组和siR-Ubc9组的细胞增殖指数分别为53.19%、54.25%和39.17%,细胞迁移距离分别为（59.47±4.66）μm、（56.56±5.37）μm和（34.57±6.61）μm,发生迁移的细胞数量分别为（89.44±8.36）个/视野、（93.84±8.79）个/视野和（41.67±5.39）个/视野,siR-Ubc9组与对照组和siR-neg组差异均有统计学意义（均P〈0.05）.对照组、siR-neg组和siR-Ubc9组的皮下肿瘤重量分别为（3.78±0.69）g、（3.72± 0.72）g和（2.09±0.61）g,细胞凋亡率分别为（7.79±2.21）%、（6.45±2.48）%,和（33.59±5.44）%,siR-Ubc9组与对照组和siR-neg组差异均有统计学意义（均P〈0.05）.对照组和siR-neg组肿瘤组织中PCNA、MMP-2和MMP-9蛋白均高表达,而siR-Ubc9组肿瘤组织中PCNA、MMP-2和MMP-9蛋白表达均低表达,差异均有统计学意义（均P〈0.05）.结论 通过沉默肝癌细胞中Ubc9基因表达能够诱导AKT1去SUMO化修饰,进而抑制肝癌细胞的增殖和转移,为未来肝癌基因治疗提供了新的借鉴方法.

双丹明目胶囊对糖尿病大鼠视网膜VEGF-a、VEGF-b、VEGF-c及其受体Flk-1表达的影响

目的:观察双丹明目胶囊对糖尿病大鼠模型视网膜血管内皮生长因子(VEGF)-a、VEGF-b、VEGF-c及其受体胎肝激酶-1(Flk-1)表达的影响。方法:将40只雄性SD大鼠,采用随机数字法分为正常组、模型组、双丹明目组、阳性对照组4组,每组10只20眼。除正常组外,其余3组大鼠采用STZ 50mg/kg的剂量一次性大鼠尾静脉注射法建立糖尿病性视网膜病变大鼠模型,造模后1周后开始连续灌胃用药,灌胃后8周,处死动物,免疫组化法检测视网膜组织中VEGF-a、VEGF-b、VEGF-c及其受体Flk-1的表达。结果成模后用药第8周,模型组、双丹明目组、阳性对照组视网膜中VEGF-a、VEGF-b、VEGF-c及其受体Flk-1蛋白表达平均光密度均高于正常组,其中模型组与正常组比较,差异有统计学性意义(P<0.01);双丹明目组、阳性对照组VEGF-a、VEGF-b、VEGF-c及其受体Flk-1表达的平均光密度值均低于模型组(P<0.01)。结论:双丹明目胶囊能明显降低VEGF-a、VEGF-b、VEGF-c及其受体Flk-1在糖尿病模型大鼠视网膜中的表达,对其视网膜有一定的保护作用。

白芦藜醇通过抑制血管内皮生长因子受体-1-磷脂酰肌醇3激酶/蛋白激酶B信号转导通路影响HepG2细胞增殖

目的观察白芦藜醇通过抑制血管内皮生长因子受体(VEGFR)-1-磷脂酰肌醇3激酶(PI3K)/蛋白激酶B(Akt)信号转导通路对肝癌细胞增殖的影响。方法采用噻唑蓝(MTT)法检测白芦藜醇对HepG2细胞(2017年6月购自上海普诺赛生物)细胞增殖的抑制作用,流式细胞术检测细胞周期变化,反转录-聚合酶链反应(RT-PCR)检测VEGFR-1、Akt基因表达水平,蛋白质印迹法(Western blot)检测磷酸化(p)-VEGFR-1、VEGFR-1、p-Akt和Akt表达水平。采用转化后的Cochran Armitage趋势检验。结果白藜芦醇对HepG2细胞增殖具有明显的抑制作用,且呈剂量和时间依赖性,表明白藜芦醇浓度增加,作用时间越长,对HepG2细胞增殖的抑制作用越强。白藜芦醇浓度为0、20、80、160μmol/L时G0/G1分别为35.60、40.91、49.35和55.15,结果显示白藜芦醇作用HepG2细胞48 h后,可使肝癌HepG2细胞周期阻滞于G0/G1期。白藜芦醇浓度由5μmol/L逐渐增加至160μmol/L时,HepG2细胞中VEGFR-1表达水平由1.00±0.08逐渐降至0.28±0.02。HepG2细胞中Akt mRNA表达水平由2.32±0.22逐渐降至1.08±0.10。随着白藜芦醇浓度的增加,HepG2细胞中p-VEGFR-1、VEGFR-1、Akt和p-Akt蛋白表达水平均显著降低(χ2=15.183、17.842、32.628、26.163,P<0.05),其随白藜芦醇浓度变化而变化的趋势,经Cochran Armitage趋势检验,差异均有统计学意义(χ2=22.798,P<0.05)。结论白芦藜醇通过抑制VEGFR-1-PI3K/Akt信号转导通路的表达可抑制肝癌HepG2细胞增殖。

内毒素耐受大鼠肝组织白细胞介素－1受体相关激酶－4和相关激酶－M的表达及其意义

目的探讨内毒素耐受（ETT）大鼠肝组织IL-1受体相关激酶（IRAK）－4和IRAK—M的表达变化及其意义。方法将66只雄性SD大鼠分为对照组、急性肝功能衰竭（ALF）组和ETT组。ETT组腹腔注射脂多糖（LPS），ALF组注射等量0．75％氯化钠溶液，然后ETT组与ALF组同时腹腔注射D-氨基半乳糖（D-GaIN）及LPS，在注射后2、6、12、24和48h时间点留取大鼠血液及肝脏标本。观察肝组织的病理变化，ELISA法检测TNF-α及IL-6水平，RT—PCR检测IRAK-4、IRAK—M、核因子-κB（NF-κB）（p65）mRNA表达情况。统计学处理采用LSD检验和Dunnet’s t检验。结果ETT组大鼠肝组织病理改变明显轻于ALF组。在2、6、12、24、48h，ALF组大鼠肝组织IRAK-4 mRNA／β-肌动蛋白（β-actin）吸光度比值分别为0．711±0．074、0．904±0．118、1．012±0．098、1．534±0．279、1．451±0．290，IRAK—M mRNA／β-actin吸光度比值分别为0．496±0．018、0．516±0．089、0．503±0．023、0．503±0．057、0．469±0．142；ETT组IRAK—M mRNA／β—actin吸光度比值分别为0．929±0．064、1．111±0．138、1．113±0．027、1．891±0．315、1．710±0．303，IRAK-4 mRNA／β-actin吸光度比值分别为0．619±0．083、0．587±0．033、0．623±0．034、0．720±0．044、0．654±0．041。与ALF组比较，ETT组IRAK—MmRNA表达明显上升，IRAK-4mRNA表达相对降低，两组IRAK-4、NF-κB（p65）及IRAK—M在2、6、12、24、48h均差异有统计学意义（F=17．305、54．921、121．031、67．607、55．279，F=19．506、43．777、110．823、302．681、202．822，F=172．003、59．519、987．055、68．463、96．601，均P〈0．05）。结论诱导ETT可使ALF大鼠肝组织损害减轻，可能与IRAK-4表达下降、IRAK—M表达升高有关。

丹酚酸B对慢性酒精性肝损伤大鼠肝脏的保护作用

目的探讨丹酚酸B通过调控丝氨酸/苏氨酸蛋白激酶组成的异源三聚体依赖的蛋白激酶α1(AMPKα1)激活沉默信息调节因子2相关酶I(SIRT1)减轻酒精性肝损伤(ALD)的作用机制。方法用酒精液体饲料喂养建立ALD大鼠模型;另选大鼠普通饲料喂养作为空白组和对照组,将造模成功大鼠随机分为3组:模型组、低、高剂量实验组;每组均为8只。对照组、低、高剂量实验组灌胃给予丹酚酸B溶液30,15,30 mg·kg-1;空白组和模型组灌胃给予等量的0.9%NaCl,连续给药8周。用试剂盒检测丙氨酸氨基转移酶(ALT)水平。用蛋白免疫印迹法(Western Blot)检测大鼠肝脏组织SIRT1、AMPKα1及p-AMPKα1的蛋白表达情况。结果空白组、对照组、模型组、低、高剂量实验组的血清ALT水平分别为(24.37±2.08),(23.09±1.02),(59.97±3.68),(43.39±2.91)和(39.08±2.17)U·L-1;SIRT1蛋白表达相对水平分别为0.60±0.02,0.75±0.03,0.13±0.02,0.20±0.01,0.27±0.01;p-AMPKα1蛋白表达相对水平分别为1.01±0.01,1.52±0.10,0.45±0.02,0.62±0.04,0.71±0.05。模型组与空白组比较,低、高剂量组与模型组比较,上述指标的差异均有统计学意义(均P<0.01)。结论丹酚酸B通过调控AMPKα1磷酸化水平激活SIRT1蛋白表达,进而发挥其抗慢性酒精性肝病的保护作用。