Cloning and Sequence Analysis of HN and F Protein Genes from a Strain of Goose Paramyxovirus

[ Objective] The study was to clone HN and F genes from GX1 strain of goose paramyxovirus and analyze their sequences. [ Method] According to the full nucleotide sequence of GPV-SF02 strain of goose paramyxovirus, two pairs of pdmers were designed to amplify the HN and F genes from GX1 strain of goose paramyxovirus isolated from diseased goose in Guangxi Zhuang Autonomous Region; the amplified products were ligated into pMD18-T vector and sequenced. [ Result ] HN and F genes of this strain tested were 1 716 and 1 662 bp in full nucleotide length, respectively; both showed the homologues of about 97.3% with GPV- SF02 strain, of 80.3% -97.5% with strains LaSota, F48E9 and JS, of just 84.8% with Miyadera strain. [ Conclusion] The results show that isolated strain BX1 matches to virulent APMV-1 strain, belonging to genotype Ⅶ of APMV-1 strain.

Screening of hepatocyte proteins binding to F protein of hepatitis C virus by yeast two-hybrid system

AIM： To investigate the biological function of F protein by yeast two-hybrid system. METHODS： We constructed F protein bait plasmid by cloning the gene of F protein into pGBKT7, then recombinant plasmid DNA was transformed into yeast AH109 （a type）. The transformed yeast AH109 was mated with yeast Y187 （α type） containing liver cDNA library plasmid in 2×YPDA medium. Diploid yeast was plated on synthetic dropout nutrient medium （SD/-Trp-Leu-HisAde） containing X-α-gal for selection and screening. After extracting and sequencing plasmids from positive （blue） colonies, we underwent sequence analysis by bioinformatics. RESULTS： Thirty-six colonies were selected and sequenced. Among them, 11 colonies were zymogen granule protein, 5 colonies were zinc finger protein, 4 colonies were zinc-α-2-glycoprotein, 1 colony was sialyltransferase, 1 colony was complement control protein factor I, 1 colony was vitronectin, and 2 colonies were new genes with unknown function. CONCLUSION： The yeast two-hybrid system is an effective method for identifying hepatocyte proteins interacting with F protein of hepatitis C virus. F protein may bind to different proteins. 2005 The WJG Press and Elsevier Inc. All rights reserved

Cloning and expression of special F protein from human liver

AIM： To clone human liver special F protein and to express it in a prokaryotic system. METHODS： Total RNA was isolated from human liver tissue and first-strand cDNA was reverse transcribed using the PCR reverse primer. Following this, cDNA of the F protein was ligated into the clone vector pUCm-T. The segment of F protein＇s cDNA was subdoned into the expression vector pET-15b and transformed into E. coli BL21 （DE3） pLyss. Isopropy-β-D-thiogalactoside （IPTG） was then used to induce expression of the target protein. RESULTS： The cDNA clone of human liver special F protein （1134bp） was successfully produced, with the cDNA sequence being published in Gene-bank： DQ188836. We confirmed the expression of F protein by Western blot with a molecular weight of 43 kDa. The expressed protein accounted for 40% of the total protein extracted. CONCLUSION： F protein expresses cDNA clone in a prokaryotic system, which offers a relatively simple way of producing sufficient quantities of F protein and contributes to understanding the principal biological functions of this protein.

Construction of Recombinant Expression Plasmids Containing H and F Protein Genes of Canine Distemper Virus Isolated from a Mink and Their Expression in Prokaryotic Cells

[Objective] This study aimed to construct the recombinant expression plasmids containing H and F protein genes of Canine distemper virus isolated from a mink and to express these two genes in prekaryotic cells as well as to study the reactogenieity of the expressed products. [ Method ] RT-PCR amplification was used to obtain H and F protein genes; TA cloning and subclonlng techniques were used to construct the cloning plasmids（pMD-18T-H and pMD-18T-F） and recombinant expression plasmids（pET28a-H and pET28a-F） ; SDS-PAGE and Western-blotting were adopted to verify whether the target proteins were successfully expressed. [ Result] The recombinant expression plasmids pET28a-H and pET28a-F containing H and F protein genes of Canine distemper virus isolated from a mink were successfully constructed, and both the expressed H and F proteins with respectively relative molecular mass of 31 400 and 38 200 produced positive reac- tion with the CDV standard positive serum. [ Conclusion] The H and F proteins expressed in prokaryotic cells were the same with the natural ones in terms of reac- togenicity, which can be utilized for diagnosis of a CDV＇s infection or for an epidemiological investigation. Meanwhile, they also provide a basis for developing ge- netically engineered subunit vaccines.

血清抗着丝粒蛋白F抗体在乳腺癌中的临床价值探讨

目的:探讨血清抗着丝粒蛋白F抗体(anti-centromere protein F antibody,anti-CENPF)在乳腺癌中的临床价值。方法:收集100例初诊乳腺癌(breast cancer,BC)患者、40例乳腺良性疾病(non breast cancer,non-BC)患者和40名健康体检者(healthy control,HC)血清,采用酶联免疫吸附试验检测血清中的anti-CENPF水平,同时化学发光法测定血清糖类抗原153(carbohydrate antigen 153,CA153)的水平。结果:BC组血清anti-CENPF水平高于non-BC组和HC组,差异有统计学意义(P<0.05)。anti-CENPF和CA153诊断乳腺癌中的曲线下面积(area under the curve,AUC)分别为0.714和0.672,两者联合检测的AUC为0.739。有淋巴结转移、远处转移或者人表皮生长因子受体2(human epidermal growth factor receptor-2,HER-2)阴性的乳腺癌患者血清anti-CENPF浓度明显升高(P<0.05)。不同肿瘤大小、临床分期、分子分型乳腺癌患者血清anti-CENPF水平比较,差异有统计学意义(P<0.05)。组间比较显示Ⅳ期和Ⅲ期血清anti-CENPF浓度高于Ⅰ期和Ⅱ期,HER-2过表达型、Luminal B型血清anti-CENPF水平低于三阴性乳腺癌(triple negative breast cancer,TNBC)患者。雌激素受体(receptors estrogen,ER)阳性的乳腺癌患者中,HER-2阴性组的anti-CENPF浓度高于HER-2阳性组,差异有统计学意义(P=0.026)。结论:血清antiCENPF在乳腺癌的诊断、临床分期及分子分型中发挥了重要作用,其水平可能与乳腺癌预后呈负相关,有望成为乳腺癌潜在的疾病标志物。

牛呼吸道合胞体病毒G和F蛋白的生物学功能

牛呼吸道合胞体病毒(bovine respiratory syncytial virus, BRSV)是一种在世界范围内引起牛呼吸道疾病的病毒性病因之一,主要引起1岁龄以下犊牛的严重下呼吸道感染。BRSV共编码9种结构蛋白,其中附着蛋白(G蛋白)和融合蛋白(F蛋白)是BRSV表面主要的包膜糖蛋白,参与病毒吸附、融合宿主细胞的过程。G和F蛋白含多种识别表位,能够刺激机体产生中和抗体反应,常常是牛呼吸道合胞体病(bovine respiratory syncytial disease, BRSD)疫苗开发所关注的重点。探究G和F蛋白在BRSV侵染中的作用机理对于病毒致病机理分析、疫苗开发具有重要意义。本文旨在对牛呼吸道合胞体病毒G和F蛋白的结构功能及有关疫苗的开发加以综述,以期为BRSV疫苗的研制和BRSD的防控提供参考。

着丝粒蛋白F、miR-1-3p在中晚期胃癌患者血清中的表达及与预后的相关性

目的探讨着丝粒蛋白F(CENPF)、miRNA-1-3p(miR-1-3p)在中晚期胃癌患者血清中的表达及与预后的相关性。方法选取2019年3月至2020年3月我院收治的60例中晚期胃癌患者即为研究组,同期在我院体检中心体检健康的志愿者60例为对照组。采用实时荧光定量PCR(qRT-PCR)法检测各组血清CENPF、miR-1-3p的表达水平;采用Pearson法分析血清中CENPF、miR-1-3p水平的相关性;采用Kaplan-Meier法分析CENPF、miR-1-3p表达与中晚期胃癌患者预后的关系;COX回归分析影响中晚期胃癌患者预后的危险因素。结果与对照组比较,研究组患者CENPF水平明显升高,miR-1-3p水平明显降低(P<0.05)。相关性分析结果显示,中晚期胃癌患者血清中CENPF和miR-1-3p水平呈负相关(r=-0.650,P<0.001)。不同TNM分期和淋巴结转移状况下CENPF、miR-1-3p水平比较差异有统计学意义(P<0.05)。CENPF高表达组患者3年生存率63.33%(19/30)显著低于低表达组93.33%(28/30)(χ^(2)=7.954,P<0.001);miR-1-3p高表达组患者3年生存率96.67%(29/30)显著高于低表达组60.00%(18/30)(χ^(2)=11.882,P=0.001)。多因素COX回归分析显示,TNM分期、淋巴结转移、CENPF、miR-1-3p表达是影响中晚期胃癌患者预后的危险因素(P<0.05)。结论中晚期胃癌患者血清中CENPF水平显著升高,miR-1-3p水平显著降低,二者与预后有关。

新城疫病毒F蛋白和禽致病性大肠杆菌OmpA嵌合蛋白的表达及双特异性抗体制备

为获得Ⅶ型新城疫病毒(Newcastle disease virus,NDV)融合蛋白(fusion protein,F蛋白)和O18型禽致病性大肠杆菌(avian pathogenic Escherichia coli,APEC)外膜基因A(outer-membrane proteases,OmpA)嵌合蛋白和双特异性抗体,试验首先采用基因合成技术获得Ⅶ型NDV F基因和O18型APEC的OmpA基因片段,使用同源重组技术将F基因插入到OmpA基因中,再将重组基因片段插入到原核表达载体pGEX-4T-1中构建嵌合表达质粒,对重组质粒中的插入基因序列进行测序鉴定;将序列正确的嵌合表达质粒转入大肠杆菌BL21(Rosetta)感受态细胞中,利用IPTG诱导嵌合蛋白表达,使用SDS-PAGE和Western-blot检验嵌合蛋白的表达情况;纯化嵌合蛋白后免疫兔获得抗血清,抗血清再经抗原亲和纯化层析柱纯化获得多克隆抗体,采用间接酶联免疫吸附试验(enzyme linked immunosorbent assay,ELISA)测定抗体效价。结果表明:成功合成了Fo和OmpA1、OmpA2基因片段,构建并表达了重组质粒pGEX-O1-Fo-O2,纯化后的嵌合蛋白O1FoO2在大肠杆菌中以包涵体形式存在,制备的多克隆抗体对O1FoO2的效价约为1.1×10^(6),对GST的效价约为4.1×10^(4)。说明制备的嵌合蛋白和双特异性抗体质量较好。

前列腺癌组织中硒结合蛋白1、硒蛋白F表达与患者临床病理特征及预后的关系研究

目的研究前列腺癌(PC)组织中硒结合蛋白1(SELENBP1)、硒蛋白F(SELENOF)表达与患者临床病理特征关系和预后的关系。方法选取2017年1月至2020年1月邯郸市中心医院诊治的104例PC患者作为研究对象。检测PC患者癌组织和癌旁组织中SELENBP1、SELENOF表达水平,并分析两者与PC患者临床病理特征和预后的关系。采用多因素COX回归分析影响PC患者预后的因素。结果PC患者癌组织中SELENBP1、SELENOF阳性率低于癌旁组织(P<0.05)。不同Gleason评分、TNM分期及术前前列腺特异性抗原(PSA)水平的PC患者癌组织中SELENBP1、SELENOF阳性率比较,差异具有统计学意义(P<0.05)。SELENBP1阴性患者、SELENOF阴性患者3年无进展生存率分别低于SELENBP1阳性患者、SELENOF阳性患者(P<0.05)。TNM分期Ⅲ期、Gleason评分>7分、SELENBP1阴性、SELENOF阴性是影响PC患者预后的独立危险因素(P<0.05)。结论PC患者癌组织中SELENBP1、SELENOF表达降低,且两者与PC患者不良临床病理特征相关,可导致PC患者不良预后。

CENPF调控PI3K/AKT信号通路影响唾液腺腺样囊性癌进展

目的:探讨着丝粒蛋白F(centromere protein F,CENPF)在腺样囊性癌(adenoid cystic carcinoma,ACC)发生发展中的作用和分子机制。方法:通过小干扰RNA转染敲低ACC细胞中的CENPF。通过细胞计数试剂盒(cell counting kit-8,CCK-8)、划痕实验和Transwell测定评估敲低CENPF对ACC细胞增殖、迁移、侵袭的影响;通过蛋白免疫印迹实验分析改变CENPF表达后ACC细胞中磷脂酰肌醇-3-激酶(phosphatidylinositol-3-kinase,PI3K)/丝氨酸/苏氨酸蛋白激酶(serine/threonine protein kinase,AKT)/哺乳动物雷帕霉素靶蛋白(mammalian target of rapamycin,mTOR)信号通路相关蛋白表达变化,通过CCK-8、划痕实验和Transwell测定评估敲低CENPF联合PI3K抑制剂BKM-120对ACC细胞增殖、迁移、侵袭的影响。结果:敲低ACC-M中CENPF表达后,CCK-8实验证明其增殖能力减弱;划痕实验表明其迁移能力减弱,Transwell实验表明其侵袭能力减弱,PI3K/AKT通路关键蛋白p-PI3K、p-AKT和p-mTOR蛋白表达水平下降。在下调CENPF的ACC-M中加入PI3K抑制剂,PI3K/AKT通路关键蛋白表达水平进一步下降。此外,加入PI3K抑制剂后,CENPF下调的ACC-M增殖、迁移、侵袭能力较单纯下调CENPF的ACC-M进一步减弱。结论:CENPF通过调控PI3K/AKT信号通路参与ACC进展。

RhoF介导的Th17极化在急性胰腺炎发生中的作用及机制

目的探讨Rho相关GTP结合蛋白F(RhoF)介导的Th17极化在重度急性胰腺炎(SAP)发生中的作用及机制研究。方法将RhoF转基因小鼠随机分为3组:对照组(n=10)、SAP组(n=10)和SAP+Y-27632组(n=10)。另将WT小鼠随机分为3组:对照组(n=10)、SAP组(n=10)和SAP+Y-27632组(n=10)。除对照组外,其他组建立SAP模型。SAP+Y-27632组在模型建立后,通过尾静脉输注Y-27632。分离小鼠血液样本中的T细胞,用于RhoF、p-MYPT1蛋白检测和ROCK活性测定,并采用流式细胞仪分析产生IL-17的淋巴CD4+T细胞的百分比。结果与对照组相比,SAP组小鼠T细胞中RhoF、p-MYPT1表达量增加(P<0.01),并且RhoF的水平与p-MYPT1的水平密切相关(P<0.05)。与WT组相比,RhoF组小鼠T细胞的RhoF蛋白水平的表达增加约30%,并且CD4+T细胞自发产生IL-17的水平显著增加(P<0.01)。与WT小鼠相比,RhoF转基因小鼠胰腺损伤的组织学评分,T细胞的RhoF、p-MYPT1表达量,IL-17+T细胞数量和血清IL-17水平明显增加(P<0.05)。SAP+Y-27632组的组织学评分,T细胞的RhoF、p-MYPT1表达量,IL-17+T细胞数量和血清IL-17水平显著低于SAP组(P<0.05)。结论RhoF/ROCK信号通路介导的Th17细胞极化参与SAP的发病机制。

1-Methyl-4-phenyl-pyridinium time-dependently alters expressions of oxoguanine glycosylase 1 and xeroderma pigmentosum group F protein in PC12 cells

Objective To determine if DNA excision repair enzymes oxoguanine glycosylase 1 （OGG1） and xeroderma pigmentosum group F protein （XPF） are involved in the pathogenesis of Parkinson＇s disease （PD） in a cell model. Methods PC12 cells were treated with 1-Methyl-4-phenylpyridine ion （MPP＋） for various periods of time to induce oxidative DNA damage. MTT assay was used to determine cell viability. Immunocytochemistry with antibody against 8-hydroxy-2＇- deoxyguanosine （8-oxodG） was used to evaluate oxidative DNA damage. Immunoblotting was used to detect the protein levels of OGG1 and XPF. Results MPP＋ treatment （1 mmol/L） for 18 h and 24 h reduced cell viability to 78.6% and 70.3% of the control, respectively, in a time-dependent way. MPP＋ increased the immunoreactivity of 8-oxodG in the cytoplasm at 3 h and in the nucleus at 24 h of treatment. With the treatment of MPP＋, the expression of OGG1 was significantly increased at 1 h, reaching a peak at 3 h, and then it was decreased at 24 h, as compared to that with vehicle treatment. The same effect was exerted on XPF level, except that the XPF level reached a peak at 18 h of MPP＋ treatment. Moreover, the maximally-increased protein level of OGG1 by MPP＋ was approximately 2-fold higher than that of XPF. Conclusion MPP＋ treatment could time- dependently induce increases in OGG1 and XPF expressions in PC12 cells. Also, this study indicates that the base and nucleotide excision repair pathways may be compensatorily activated in the early stage of pathogenesis in the cells after MPP＋ treatment.

FBXW7/MCM7信号轴介导肝癌细胞增殖的研究

目的 探讨FBXW7靶向调控MCM7表达对肝癌细胞增殖的影响。方法 采用免疫共沉淀法(CoIP)和免疫荧光染色法(IF),分析肝癌细胞系MHCC-97H中FBXW7与MCM7的互作关系;通过慢病毒感染过表达FBXW7和(或) MCM7,小干扰RNA技术下调FBXW7和(或) MCM7的表达;采用Western blot检测FBXW7对MCM7蛋白表达的影响,CCK-8实验检测肝癌细胞的增殖活性,EdU细胞增殖检测分析肝癌细胞的增殖能力,平板克隆实验分析肝癌细胞的集落形成能力。结果 在MHCC-97H细胞中,FBXW7与MCM7存在互作关系:过表达FBXW7抑制了MCM7的蛋白表达水平、并抑制了肝癌MHCC-97H细胞的增殖(P <0.05),在过表达FBXW7的基础上增加MCM7的表达后,细胞增殖能力提高(P <0.05);下调FBXW7后细胞中MCM7表达增加、细胞增殖能力增强(P <0.05),而下调FBXW7的同时干扰MCM7表达后,细胞增殖能力减弱(P <0.05)。结论 FBXW7能抑制肝癌细胞增殖,其机制与负向调节肝癌细胞中促癌蛋白MCM7的表达水平有关。

Genetic Characterization of Fusion Protein of Human Respiratory Syncytial Virus: Beijing

Objective Fusion protein is a subunit of the human respiratory syncytial virus(HRSV)and a potential vaccine candidate.Thus,a study on the genetic characteristics of F protein was considered important for further investigations in this field.The aim of this study was to determine the prevalence and genetic diversity of the F gene of HRSV infections in hospitalized pediatric patients in Beijing with acute lower respiratory tract infections and to compare the circulating genotypes that are currently found worldwide.Methods HRSV particles were amplified by RT-PCR and the PCR products were purified for sequencing.Further analysis was carried out by Bioedit and MEGA 3.0 biological software programs.Results Seventy-six samples(23.1%)were positive for HRSV.The percentage of cases in patients younger than 1year was 84.21%.Among the six Beijing isolates,four belonged to subgroup A,whose respective F genes shared97.0%-97.4%nucleotide sequence identity and 92.1%-93.0%amino acid sequence identity.The other two isolates belonged to subgroup B.Here,97.3%and 98.2%sequence identity were found at nucleotide and amino acid levels,respectively.Conclusions Phylogenetic analysis of nucleotide sequences revealed that those four isolates within subgroup A were monophyletic and closely related to each other,but those two within subgroup B distributed in two distinct clusters.Subgroup A and B strains co-circulated,indicating that two different transmission chains occurred in Beijing from 2003-2004.

^(18)F-FAPI-42的自动化合成及小动物PET/CT显像研究

成纤维细胞活化蛋白(fibroblast activation protein,FAP)在多数上皮来源恶性肿瘤中高度表达,FAP抑制剂(FAPI)经核素标记后已用于肿瘤的早期诊断。为实现PET显像剂^(18)F-FAPI-42的自动化合成并进行质量控制,本研究基于Allinone合成器及其配套的空白试剂盒,通过一锅反应自动化制备^(18)F-FAPI-42,并在荷胶质母细胞瘤U87-MG模型鼠行小动物PET/CT(positron emission tomography/computed tomography)动态显像对其进行评价。结果显示,^(18)F-FAPI-42的自动化合成时间在60 min以内,放化产率为(15.8±3.2)%(n=10,未经衰变校正),放化纯度>95%,比活度14~52 GBq/μmol。小动物PET/CT动态显像显示,^(18)F-FAPI-42对肿瘤显影清晰,放射性滞留时间长,具有较高的肿瘤与肌肉摄取比,活度与时间曲线显示其主要通过肾脏排泄。以上结果表明,Allinone合成器能够稳定高效地合成符合药物质控标准的^(18)F-FAPI-42,所得产品质量满足临床要求。该合成方法可为NOTA类修饰化合物的^(18)F标记提供参考和借鉴。

犬瘟热病毒F蛋白融合信号肽单克隆抗体的制备及其表位的鉴定

为制备犬瘟热病毒(CDV)F蛋白融合信号肽(FSP)的单克隆抗体(MAb),本研究通过原核表达系统表达CDV HLJ1-13株重组FSP蛋白(rFSP)。将其免疫BALB/c小鼠,通过间接ELISA方法筛选到1株能够稳定分泌抗FSP蛋白MAb的杂交瘤细胞株G8D6E3E5,亚类鉴定结果显示该株MAb重链为Ig G2a型,轻链为κ型。构建一系列表达部分重叠的重组FSP片段,经western blot鉴定该株MAb识别的抗原区域为aa1~aa55,通过合成一系列重叠多肽,经ELISA进一步鉴定该株MAb识别的抗原表位为^(21)QQHSTRSTET^(30)。采用western blot检测该株MAb与r FSP的反应原性;采用间接免疫荧光试验(IFA)检测该株MAb与天然FSP的反应原性。Western blot结果显示,CDV Snyder Hill和HLJ1-13株r FSP蛋白样品在34 ku左右均出现特异性条带;IFA结果显示,感染CDV Snyder Hill株48 h后的vero细胞出现红色荧光。以上结果表明,该株MAb既能够与原核表达的CDV Snyder Hill和HLJ1-13株的r FSP蛋白反应,也能够与天然表达的CDV Snyder Hill株FSP蛋白反应。上述研究结果为CDV的检测以及FSP生物学功能的研究奠定了坚实基础。

表达呼吸道合胞病毒融合前F蛋白的重组人5型腺病毒的构建

目的筛选并构建成功表达A亚型人呼吸道合胞病毒(Human Respiratory Syncytial Virus,HRSV)融合前构象F蛋白的重组人5型腺病毒(Recombinant Human type5 adenovirus,rHADV-5),为制备和研发HRSV重组腺病毒载体疫苗奠定基础。方法在真核表达载体pcDNA3.1(+)上插入具有不同突变位点的HRSV F蛋白编码序列,利用融合前F蛋白单克隆抗体AM14和D25筛选HRSV F蛋白突变体;通过同源重组将筛选出的前构象F蛋白突变体编码序列插入非复制型人5型腺病毒载体,在HEK293细胞中进行重组病毒的包装和扩增,经氯化铯密度梯度法获得纯化的重组病毒;应用夹心ELISA法和Western blot鉴定F蛋白的表达及构象。结果通过AM14和D25单克隆抗体筛选出了2个稳定维持在融和前构象的HRSV F蛋白序列(SC-3M和SC-5M)。将SC-3M和SC-5M编码序列插入非复制型人5型腺病毒载体,对两种重组人5型腺病毒(pAd5-SC-3M和pAd5-SC-5M)和空载体(pAd5-vector)纯化,病毒滴度分别达到2.016×10^(10),2.52×10^(10)和2.948×10^(11)IU/mL。pAd5-SC-3M和pAd5-SC-5M感染HEK293后均能高效表达HRSV融合前构象的F蛋白并维持三聚体结构,且pAd5-SC-5M感染细胞中F蛋白表达量高于pAd5-SC-3M。结论成功在体外传代细胞中获得可高效表达A型HRSV融合前F蛋白的重组人5型腺病毒,为进一步通过动物试验评价该HRSV重组腺病毒载体疫苗奠定了基础。

FBXL2和Dkk-1在结直肠癌组织中的表达及临床意义

目的研究结直肠癌(CRC)组织中F-盒富含亮氨酸的重复蛋白2(FBXL2)、Wnt信号通路抑制剂1(Dkk-1)的表达及临床意义。方法选取2017年10月—2019年5月保定市第一中心医院普通外科诊治CRC患者75例作为研究对象。应用荧光定量PCR及免疫组化检测CRC癌组织和癌旁组织中FBXL2、Dkk-1 mRNA及蛋白表达水平。比较不同临床病理特征CRC患者癌组织中FBXL2、Dkk-1蛋白表达差异。Kaplan-Meier生存分析(Log-rank检验)FBXL2、Dkk-1蛋白表达与CRC患者生存预后的关系。多因素COX回归分析影响CRC患者生存预后的危险因素。结果CRC癌组织中FBXL2、Dkk-1 mRNA表达水平低于癌旁组织(t=25.053、34.053,P均<0.001)。CRC癌组织中FBXL2、Dkk-1蛋白表达阳性率低于癌旁组织(χ^(2)=58.134、51.042,P均<0.001)。CRC癌组织中FBXL2与Dkk-1蛋白表达呈显著正相关(r s=0.714,P<0.001)。TNM分期Ⅰ~Ⅱ期、淋巴结转移阴性CRC患者癌组织中FBXL2、Dkk-1蛋白表达阳性率高于TNM分期Ⅲ期、淋巴结转移阳性患者,差异均有统计学意义(χ^(2)/P=7.588/0.006、5.220/0.022)。FBXL2阴性表达组患者3年累积生存率明显低于阳性表达组患者(χ^(2)=5.991,P=0.014);Dkk-1阴性表达组患者3年累积生存率明显低于阳性表达组患者(χ^(2)=8.058,P=0.005)。肿瘤分期Ⅲ期、淋巴结转移阳性、FBXL2阴性表达、Dkk-1阴性表达是影响CRC患者预后的独立危险因素[HR(95%CI)=1.613(1.223~2.126),1.917(1.314~2.799),1.837(1.229~2.745),1.738(1.246~2.426),P均<0.001]。结论CRC癌组织中FBXL2、Dkk-1表达降低,两者表达与CRC肿瘤分期及淋巴结转移有关,是评估CRC患者生存预后新的肿瘤标志物。

着丝粒蛋白F在胶质瘤组织中的表达及预后分析

目的探究着丝粒蛋白F(CENPF)在脑胶质瘤中的表达及预后分析。方法通过对癌症基因组图谱(TCGA)和中国脑胶质瘤图谱(CGGA)数据库进行生物信息分析,比较CENPF在低级别胶质瘤(LGG)、胶质母细胞瘤(GBM)和癌旁组织中的表达差异以及与患者预后之间的关系,并在数据库中对CENPF mRNA与P53、Ki-67以及IDH-1分型进行相关性分析。采用实时荧光定量PCR(qRT-PCR)法检测CENPF mRNA表达水平,免疫组织化学法和Western blotting法检测癌旁组织和不同级别胶质瘤组织中CENPF表达水平。多因素COX分析CENPF与临床病理参数及患者预后的关系,并绘制Kaplan-Meier生存曲线。利用TCGA数据库对CENPF进行KEGG富集分析,探索该基因在胶质瘤中发展中可能参与的信号通路。结果CENPF表达水平与胶质瘤WHO分级呈正相关,且CENPF高表达的胶质瘤患者生存时间短于低表达患者。数据库相关性分析显示CENPF mRNA与P53、Ki-67以及IDH-1野生型呈正相关。qRT-PCR实验结果表明CENPF mRNA在胶质瘤组织中表达增高,免疫组织化学和Western blotting实验结果表明CENPF表达与WHO等级呈正相关。临床病理参数分析表明在胶质瘤组织中CENPF表达情况与胶质瘤WHO分级(P=0.002)、P53(P=0.016)、Ki-67(P<0.001)表达有关。多因素COX分析显示WHO分级(P<0.001)、CENPF表达(P=0.008)、P53(P=0.003)和Ki-67(P=0.006)表达为胶质瘤患者预后不良的危险因素。Kaplan-Meier生存曲线表明CENPF高表达的胶质瘤患者生存时间短于低表达患者(P<0.0001)。KEGG富集分析显示CENPF在参与细胞周期、DNA复制、WNT/beta-catenin、mTORC1等通路中具有显著富集。结论CENPF在胶质瘤组织中表达增高,其表达与WHO分级、Ki-67以及P53分型相关;CENPF可作为判断胶质瘤患者预后的生物标志物。

FBXO38通过PI3K-Akt信号通路调控眼部黑色素瘤增殖

目的·研究F-box蛋白38(F-box only protein 38,FBXO38)对眼部黑色素瘤增殖的作用以及潜在的调控通路。方法·使用FBXO38短发夹RNA(short hairpin RNA,shRNA)和FBXO38过表达质粒构建FBXO38敲低以及过表达的人皮肤黑色素瘤A375和葡萄膜黑色素瘤OMM2.3细胞系,并通过实时荧光定量PCR(quantitative real-time PCR,qRT-PCR)和Western blotting在转录和蛋白水平验证FBXO38的敲低和过表达效率。通过克隆形成实验、BrdU免疫荧光染色和CCK8细胞增殖实验,探究FBXO38对黑色素瘤细胞增殖的影响。使用肿瘤基因组图谱计划数据库(The Cancer Genome Atlas,TCGA),分析FBXO38高表达和低表达组中的差异表达基因,并进行京都基因与基因组数据库(Kyoto Encyclopedia of Genes and Genomes,KEGG)通路富集,揭示与FBXO38相关的信号通路。进一步通过CCK8细胞增殖实验检测信号通路抑制剂对不同FBXO38表达量细胞的抑制率。同时通过qRT-PCR和Western blotting,验证在敲低FBXO38之后该通路是否激活。结果·qRT-PCR和Western blotting验证A375和OMM2.3细胞系中的FBXO38的mRNA及蛋白质表达水平,发现与对照组相比敲低组的FBXO38表达水平下降,与野生型相比过表达组的FBXO38的表达水平提高(P<0.05)。克隆形成实验、BrdU免疫荧光染色和CCK8细胞增殖实验显示,敲低FBXO38显著增强A375和OMM2.3细胞的增殖能力(P<0.05),反之过表达FBXO38抑制A375和OMM2.3细胞增殖(P<0.05)。KEGG通路富集分析显示,在皮肤黑色素瘤和葡萄膜黑色素瘤中,FBXO38的表达影响磷脂酰肌醇3激酶/蛋白激酶B(phosphoinositide 3-kinase/protein kinase B,PI3K-Akt)通路激活。与对照组相比,PI3K抑制剂LY294002和mTOR1抑制剂Everolimus对FBXO38敲低组的抑制率显著提升(P<0.05),对FBXO38过表达组的抑制率则显著下降(P<0.05)。Western blotting结果显示,敲低FBXO38之后,与PI3K-Akt通路相关的PTEN、P21和P53蛋白水平下降,而MDM2蛋白水平上升。qRT-PCR结果显示在FBXO38敲低细胞中P53转录水平显著下降(P<0.05),而MDM2转录水平显著上升(P<0.05)。结论·FBXO38通过PI3K-Akt信号通路参与调控眼部黑色素瘤细胞的增殖。