垂体瘤转化基因1(PTTG1)的表达变化对人前列腺癌细胞LNCaP生长增殖的影响

垂体肿瘤转化基因1(PTTG1)具有促进肿瘤生长和转移的作用.通过上调或下调基因表达的策略,观察PTTG1基因对人前列腺癌细胞株LNCaP细胞生长增殖的影响.利用PCR技术分离出PTTG1全长cDNA,分别正向和反向插入真核表达载体pIRES2-EGFP,重组载体分别命名为正义PTTG1-S/pIRES2-EGFP(即pI-P-S)和反义PTTG1-AS/pIRES2-EGFP(即pI-P-AS),将这两种重组载体稳定转染LNCaP细胞,通过流式细胞仪和MTT法分别检测了细胞周期和细胞增殖的情况.转染正义PTTG1后处于S期和G2期的细胞明显增加,细胞生长增殖能力增强;相反,转染反义PTTG1后处于S期和G2期细胞明显减少,细胞生长增殖能力减弱(P<0.05).结果表明,PTTG1能明显改变人前列腺癌细胞株LNCaP的细胞周期和细胞生长增殖能力,它的异常表达可能参与前列腺癌细胞生长增殖过程.     

反义RNA抑制存活素基因的表达对HeLa细胞的影响

为研究存活素（survivin)基因在肿瘤细胞中的应用,通过RT-PCR从HeLa细胞中克隆得到存活素cDNA的编码区,将其反向克隆到可诱导型表达载体pHC中,得到存活素反义RNA表达的载体pHSC,通过脂质体的介导,将pHSC导入HeLa细胞中,经C418（800nmol/L)筛选获得可以诱导表达存活素反义RNA的稳定细胞株HeLa-pHSC。获得的细胞株在2mmol/LZn^2 的诱导下,可以表达存活素反义RNA,从而抑制存活素基因的表达,此时HeLa细胞的增殖受到抑制,对化疗药物的敏感性增加,在G2/M期可以减缓细胞周期的进行性,这表明存活素对维持肿瘤细胞的增殖以及细胞周期的进行具有非常重要的作用。     

抑癌基因NDRG2对人结肠癌细胞系Caco-2增殖的影响

目的:采用重组慢病毒系统,在过表达和抑制NDRG2 (N-myc downstream regulated gene 2)基因后,检测人结肠癌细胞系Caco-2的增殖情况.方法:分别采用NDRG2过表达慢病毒载体pLenti6-NDRG2和NDRG2干涉慢病毒载体pLKO.1-shNDRG2制备病毒并感染Caco-2细胞,经14天耐药的筛选,获得稳定感染的细胞株;采用Real time RT-PCR和Western blot方法明确NDRG2在稳转细胞株中的表达情况,同时采用MTT方法检测细胞的增殖能力,通过流式细胞仪检测细胞周期变化情况.结果:Real time RT-PCR和Western blot结果表明,在慢病毒pLenti6-NDRG2稳定感染的Caco-2细胞中,NDRG2表达上调;pLKO.1-shNDRG2稳定感染的Caco-2细胞中,NDRG2的表达下调.MTT实验结果表明,NDRG2过表达细胞株中细胞的增殖能力下降,而pLKO.1-shNDRG2慢病毒感染Caco-2后细胞的增殖能力明显增加;流式细胞术结果显示,过表达NDRG2使Caco-2细胞在G0/G1期细胞增多而S期的细胞减少,抑制细胞内源性NDRG2后G0/G1期细胞减少而S期细胞增多.结论:通过过表达和抑制NDRG2基因,验证了NDRG2作为抑癌候选基因能够有效抑制结肠癌细胞Caco-2的增殖.     

表达PKCα反义RNA对人肺癌细胞增殖的影响

 运用基因重组和基因转染技术 ,将 PKCα c DNA反向插入的重组质粒 p XJ41 - CKPα导入人肺癌 LTEPa- 2细胞 .经 Northern印迹 ,Western印迹等检验 ,表明成功地建立了稳定表达 PKCα反义 RNA的人肺癌细胞 (LT· AS4) .进一步研究了表达 PKCα反义 RNA对人肺癌细胞 LTEPa-2增殖的影响 .结果表明 ,表达 PKCα反义 RNA可抑制人肺癌细胞增殖速率 ,流式细胞光度术检测 ,G1 期细胞百分数增加 ,S期细胞百分数降低 ,并进一步探讨了其作用机理 ,观察到与增殖相关基因 c- myc、Ca M和 Cyclin B1的表达水平均下降 .这可能是 PKCα表达被阻抑、负调细胞增殖的分子机理之一     

鸟氨酸脱羧酶基因反义RNA对前列腺癌细胞生长的抑制作用

为研究鸟氨酸脱羧酶 (ODC)基因反义RNA对前列腺癌细胞的生长抑制作用 ,将表达ODC第 3外显子反义RNA的重组腺病毒rAd ODC Ex3as分别感染前列腺癌细胞株PC 3和LNCap .通过MTT法观察其对前列腺癌细胞增殖的影响 ,并确定不同细胞合适的感染滴度 ,再采用Western印迹和流式细胞术检测rAd ODC Ex3as对细胞中ODC表达的抑制作用、对细胞周期和凋亡的影响以及与CDK抑制物p2 1的关系 .实验显示 ,rAd ODC Ex3as分别以 5 0MOI、2 5MOI感染PC 3和LNCap细胞可明显抑制其生长增殖 ,而不引起细胞毒性作用 ;其对两种细胞中ODC表达的抑制作用分别为4 5 %和 5 9% .流式细胞DNA含量分析证实 ,rAd ODC Ex3as可引起PC 3和LNCap细胞周期G1期阻滞 ,但并未引起凋亡 .通过Western印迹发现 ,细胞中ODC表达的降低可诱导p2 1蛋白的过表达 .结果表明 ,rAd ODC Ex3as在体外能有效地干扰ODC基因的表达 ,并通过诱导p2 1的过表达使其细胞周期停于G1期 ,从而抑制前列腺癌细胞PC 3和LNCap的增殖 ,为其进一步基因治疗的研究打下基础 .     

LMO3过表达对胶质细胞增殖的作用

构建重组质粒pcDNA4/HisA-LMO3,转染C8-D1A胶质细胞,对照组为pcDNA4/HisA空载体质粒转染组和未转染组,MTT观察各组细胞的体外生长情况,流式细胞术(FCM)测定各组细胞的细胞周期和凋亡细胞百分比,Western-blot检测LMO3转染后凋亡相关蛋白的表达变化,从而观察LMO3基因对C8-D1A胶质细胞体外生长的影响.RT-PCR、Western印迹显示pcDNA4/HisA-LMO3转染组LMO3mRNA及LMO3蛋白表达水平明显高于对照组;与对照组细胞相比,转染组细胞的增殖能力明显高于空载体对照组及C8细胞(P0.01),S期细胞增加,G0/G1期细胞减少,C8细胞转染LMO3后可以促进C8细胞从G0/G1期进入S期,从而促进细胞的增殖.     

IL-18基因转染对大鼠C6胶质瘤细胞生长特性的影响

探讨IL-18基因转染对大鼠C6胶质瘤细胞生长特性的影响。用MTT法和流式细胞术检测C6／IL-18细胞和C6细胞的增殖特性和细胞周期分布。免疫细胞化学检测C6／IL-18细胞和C6细胞的增殖细胞核抗原(PCNA)、波形蛋白表达。结果显示,与C6细胞相比C6／IL-18细胞的增殖能力降低,G0/G1期细胞增多而G2／M期细胞减少;PCNA、波形蛋白表达降低。研究表明,IL-18基因具有抑制C6胶质瘤细胞增殖、降低其恶性程度的作用。     

BSP基因RNA干扰对乳腺癌MDA-MB-231BO细胞生物学特性的影响

旨在研究RNA干扰(RNA interference,RNAi)抑制骨唾液酸蛋白(bone sialoprotein,BSP)基因表达后对人乳腺癌细胞MDA-MB-231BO生物学特性的影响。应用pSilencer5.1-U6Retro构建针对BSP基因的siRNA逆转录病毒重组表达质粒,将重组质粒转染293细胞制备病毒悬液感染MDA-MB-231BO细胞,利用嘌呤霉素筛选抑制BSP表达的乳腺癌细胞。Western blotting检测细胞内BSP蛋白表达,采用MTT法和集落形成试验检测细胞的增殖,流式细胞仪检测细胞周期变化。结果显示,成功构建BSP基因RNAi稳定转染的231BO-BSP27细胞。231BO-BSP27细胞内BSP蛋白表达抑制率为69.3%,与对照组细胞相比,231BO-BSP27细胞的生长速率和克隆形成率明显降低;S期细胞数量明显减少,G0/G1期细胞增多。由此证实,逆转录病毒介导的RNAi能实现BSP基因稳定沉默,从而抑制MDA-MB-231BO细胞的生长和增殖。     

KAI1基因转染人乳腺癌细胞系的建立及初步研究

目的:通过将外源性KAI1基因转染入高转移性人乳腺癌细胞株,为乳腺癌基因治疗的实验室研究提供靶细胞,并初步探讨该基因对乳腺癌细胞增殖能力及细胞周期的影响。方法:采用脂质体法将pCMV-KAI1质粒转染入低表达KAIl基因的人乳腺癌细胞株MDA-MB-231中,经G418筛选后获得抗性克隆,利用RT-PCR、Western blot分析目的基因及其蛋白的表达情况,并利用MTT法和平板克隆形成实验初步探讨该基因对乳腺癌细胞体外增殖能力的影响,流式细胞术检测细胞生长周期的变化。结果:稳定转染KAI1基因的细胞株中有外源性目的基因和相应蛋白的高表达;MTT法示细胞增殖力下降,转染KAI1基因的集落形成率(25.33 2.36)％较转染前(43．17 2．75)％明显降低(P<0．05),流式细胞术显示转染KAI1基因后G1／G0期细胞数量由未转染前的(36．78 0．61)％升高至(64 7．56)％,M／G2期细胞数量则由(17．88 0．76)％降至(7．63 0．60)％,差异有显著性。结论:通过脂质体转染法获得了高表达KAI1基因及其蛋白的人乳腺癌细胞株,并发现该细胞株的体外增殖能力明显下降,这可能是KAI1基因通过调节细胞周期来实现的。     

抑癌基因NPRL2对肾癌786-O细胞增殖和凋亡的影响

抑癌基因NPRL2(nitrogen permease regulator-like 2)在人类许多正常组织中均有明显的表达,而在人类多种肿瘤组织中的表达明显降低。该实验通过构建重组质粒pEGFP-N1-NPRL2并转染肾癌786-O细胞株,应用倒置荧光显微镜、RT-PCR和Western blot检测NPRL2基因的表达情况;MTT法检测786-O细胞增殖的情况;流式细胞仪分析细胞周期和细胞凋亡情况。结果显示:肾癌786-O细胞株转染重组质粒pEGFP-N1-NPRL2后,通过荧光显微镜可以观察到绿色荧光;RT-PCR和Western blot检测到NPRL2基因的转录和蛋白质表达水平明显增加(P<0.05);MTT法检测发现72 h时pEGFP-N1-NPRL2组、pEGFP-N1组和空白对照组的细胞D490值分别为0.654±0.030、1.528±0.022和1.572±0.036,pEGFP-N1-NPRL2组细胞的增殖较其他两组受到明显的抑制(P<0.05);流式细胞仪检测显示pEGFP-N1-NPRL2组、pEGFP-N1组和空白对照组的凋亡率分别为18.82%±0.40%、5.65%±0.12%和5.85%±0.07%,而处于G0/G1期的细胞比例分别为69.80%±1.40%、46.24%±1.30%和47.03%±0.45%,与其他两组相比,pEGFP-N1-NPRL2组的凋亡率显著增高而且G0/G1期细胞明显增多,表现出G0/G1期阻滞。提示抑癌基因NPRL2的转染可以抑制786-O细胞的增殖,并诱导其凋亡将细胞周期阻滞于G0/G1期。     

Pleiotrophin stimulates fibroblasts and endothelial and epithelial cells and is expressed in human cancer.

Previously we reported the purification of the heparin-binding growth factor pleiotrophin (PTN) from supernatants of the human breast cancer cell line MDA-MB-231. To investigate further the biological activities of PTN and its potential role in cancer, we cloned a PTN cDNA and expressed the gene in a human kidney and in a human adrenal carcinoma cell line (SW-13). The supernatants harvested from cells transfected with PTN contained a heparin-binding specific protein of an apparent molecular mass of 18 kDa. These supernatants stimulated the proliferation of endothelial cells as well as the anchorage-independent growth of SW-13 cells and of normal rat kidney fibroblasts. Furthermore, SW-13 cells transfected with PTN acquired autonomous growth in soft agar and were tumorigenic in athymic nude mice. In contrast to these results with PTN from human cells, PTN obtained from insect cells (Sf9) using recombinant baculovirus as a vector was biologically inactive. We detected high levels of PTN mRNA in 16 of 27 primary human breast cancer samples (62%) as well as in 8 of 8 carcinogen-induced rat mammary tumors. Furthermore, 9 of 34 human tumor cell lines of different origin showed detectable PTN mRNA. We conclude that PTN may function as a tumor growth and angiogenesis factor in addition to its role during embryonic development.     

A colonic tissue architecture assay applied to human colon carcinoma cells

Summary A two-component tissue architecture assay system has been devised that tests the ability of human colon carcinoma cells to conform to the specific three-dimensional cell-cell and cell-substratum interactions characteristic of normal colonic tissues. Dissociated fetal rat colonic cells (FRCC) were allowed to reaggregate in suspension with or without the addition of different proportions (0.1%, 1%, and 10% of the total cells) of the human colon carcinoma cell lines, SW-1222 and LS-174T. Cellular aggregates obtained after 36 hours’ incubation exhibited cell sorting by the formation of recognizable epithelial colonic crypt-like structures with glandular lumens in a mesenchyme-like background. Carcinoembryonic antigen (CEA)-positive SW-1222 cells in 10% mixed aggregates were organized into numerous well-formed glandular structures with a polarized apical distribution of CEA. LS-174T cells, on the other hand, were self-sorted but structurally disorganized with a continuous cell surface CEA distribution. Pure FRCC and mixed aggregates were implanted under the kidney capsules of Swiss nu/nu (nude) or CD-1 nu/nu mice and allowed to grow for a period of 7–10 days. Whereas the normal FRCC readily formed colonic tissue, the SW-1222 cells exhibited a capacity for differentiation into colonic crypts which became progressively less normal and more tumor-like as the proportion of carcinoma cells in the aggregates was increased. The LS-174T cells demonstrated poor differentiation at all concentrations. Cell surface levels of CEA and the CEA family member nonspecific crossreacting antigen (NCA), both overexpressed in colon cancer, were higher in LS-174T than in SW-1222 cells, whereas family member biliary glycoprotein (BGP), downregulated in colon carcinoma was higher in the SW-1222 cells. These results thus support the suggestion that deregulated expression of CEA family members can be involved in the ability of colonocytes to differentiate and conform to normal tissue architecture as assessed by the assay. The assay is therefore amenable to genetic analysis of normal and perturbed architectural phenotypes. This work was supported by grants from the National Cancer Institute of Canada and the Medical Research Council of Canada. C. I. is a recipient of a studentship from “le Fonds pour la Formation de Chercheurs et l’Aide à la Recherche.”     

Restoration of transforming growth factor-beta type II receptor reduces tumorigenicity in the human adrenocortical carcinoma SW-13 cell line.

Transforming growth factor-beta (TGF-beta) is a potent growth suppressor. Acquisition of TGF-beta resistance has been reported in many tumors, and has been associated with reduced TGF-beta receptor expression. In this study, we examined TGF-beta 1, TGF-beta type I receptor (TbetaRI) and TGF-beta type II receptor (TbetaRII) expression in SW-13 adrenocortical carcinoma cells by Northern and Western blot analysis. SW-13 cells did not express TbetaRII mRNA or protein. We have investigated the role of TbetaRII in modulating tumorigenic potential using stably transfected SW-13 cells with TbetaRII expression plasmid. TbetaRII-positive SW-13 cell growth was inhibited by exogenous human TGF-beta1 (hTGF-beta1) in a dose-dependent manner. In contrast, SW-13 cells and control clones transfected with empty vector remained hTGF-beta1-insensitive. Xenograft examination in athymic nude mice demonstrated that TbetaRII-positive SW-13 cells reduced tumor-forming activity. Reconstructing the TbetaRII can lead to reversion of the malignant phenotype of TbetaRII-negative human adrenocortical carcinoma, which contains SW-13 cells. Reduced TbetaRII expression may play a critical role in determining the malignant phenotype of human adrenocortical carcinoma.     

Regulation of fibroblast growth factor-like protein(s) in the androgen-responsive human prostate carcinoma cell line LNCaP

Growth of the normal and malignant prostate is known to be regulated by androgens. Part of their effect has been suggested to be mediated through coordinated regulation of secreted growth factors with autocrine function. We now examine the biological role of preferentially paracrine acting factors in growth control of prostate cancer, i.e. fibroblast growth factor(s) (FGF). Coculture experiments using the androgen-responsive human prostate carcinoma cell line LNCaP as feeder cells and the FGF-dependent human adrenal carcinoma SW-13 cell line as target cells show that (i) LNCaP cells induce growth of SW-13 cells, (ii) even higher stimulation of SW-13 cells is seen in the presence of androgen treated LNCaP cells and (iii) a specific anti-bFGF antibody inhibits growth of SW-13 cells induced by androgen treated LNCaP cells; no proliferation of SW-13 cells occurs in the absence of LNCaP cells. Partial purification of the secretory products of LNCaP cells was performed by affinity chromatography using a heparin sepharose column. Fractions were tested for biological activity in a soft agar assay with SW-13 cells. Several activities could be detected, the main activity was eluted with about 1.5 M NaCl. These data suggest that androgen treatment of LNCaP cells leads to enhanced secretion of proteins which belong to the FGF-family.     

Measurement of DNA mismatch repair activity in live cells

Loss of DNA mismatch repair (MMR) function leads to the development and progression of certain cancers. Currently, assays for DNA MMR activity involve the use of cell extracts and are technically challenging and costly. Here, we report a rapid, less labor-intensive method that can quantitatively measure MMR activity in live cells. A G–G or T–G mismatch was introduced into the ATG start codon of the enhanced green fluorescent protein (EGFP) gene. Repair of the G–G or T–G mismatch to G–C or T–A, respectively, in the heteroduplex plasmid generates a functional EGFP gene expression. The heteroduplex plasmid and a similarly constructed homoduplex plasmid were transfected in parallel into the same cell line and the number of green cells counted by flow cytometry. Relative EGFP expression was calculated as the total fluorescence intensity of cells transfected with the heteroduplex construct divided by that of cells transfected with the homoduplex construct. We have tested several cell lines from both MMR-deficient and MMR-proficient groups using this method, including a colon carcinoma cell line HCT116 with defective hMLH1 gene and a derivative complemented by transient transfection with hMLH1 cDNA. Results show that MMR-proficient cells have significantly higher EGFP expression than MMR-deficient cells, and that transient expression of hMLH1 alone can elevate MMR activity in HCT116 cells. This method is potentially useful in comparing and monitoring MMR activity in live cells under various growth conditions.     

Spontaneous apoptosis of melanotic and amelanotic melanoma cells in different phases of cell cycle: relation to tumor growth

Since the spontaneous alteration of native melanotic (Ma) into amelanotic (Ab) transplantable melanoma line it has been observed that this alteration is accompanied by the acceleration of growth of Ab line. The aim of the present study was to check and estimate spontaneous apoptosis of cells from cell cycle phases. Cytometric cell cycle analysis was performed by staining cells with propidium iodide (PI). Apoptosis estimated by the TUNEL method, alterations in the plasma membrane structure (annexin V staining), changes in the mitochondrial transmembrane potential--delta psi m (JC-1 staining) showed that amelanotic melanoma cells have decreased ability to undergo spontaneous apoptosis. The obtained results showing that in the native melanotic line about 30% of cells are in S+G2/M phases and that 33% of these cells undergo apoptosis could lead to the conclusion that the slower growth of this melanoma line is the result of lower proliferation activity and higher rate of apoptosis of these tumor cells. The number of cells in S+G2/M phases in amelanotic melanoma line increases up to 40% and only 7% of them undergo apoptosis. This observation seems to suggest that the expansive growth of this melanoma line depends mainly on the decreased ability to undergo spontaneous apoptosis, especially in case of cells from S+G2/M phases. Moreover, the obtained results indicate that alteration of melanotic line into amelanotic one, accompanied by differences in many biological features also concerns basic cell processes such as cell cycle and cell death.     

p53基因对人胃癌细胞系恶性生长的影响

以p53cDNA为探针,用Southern印迹法对人胃癌细胞系BGC823进行了检测,发现该细胞中P53基因存在异常．将可在真核细胞表达的重组野生型P53质粒PC53一SN3和突变型P53质粒PC53—SCX3,用脂质体介导法,分别导入BGC823细胞,获得了较长时间耐受G418的多个阳性克隆．Southern印迹法证实阳性克隆细胞中有外源性P53基因存在．比较BGC823细胞,转染野生型及突变型P53质粒的3种细胞生长曲线和软琼脂集落形成状况发现,野生型P53基因对BGC823细胞恶性生长有一定抑制作用．     

New acceptor cell for transfected genomic DNA: oncogene transfer into a mouse mammary epithelial cell line.

A line of mouse mammary epithelial cells (NMuMG) has been characterized for its ability to be stably transfected with exogenous DNA. A transfection frequency of at least 1 cell per 1,000 was obtained with the pSV2neo plasmid. Several thousand G418-resistant NMuMG cell clones can easily be generated in cotransfection of genomic DNA and pSV2neo. The NMuMG cells were isolated from normal mammary glands and do not form malignant lesions when injected into nude mice. We have cotransfected NMuMG cells with pSV2neo and genomic DNA from the human EJ bladder carcinoma line, a cell line which contains an activated c-rasH oncogene. When a pool of 4,700 G418-resistant colonies was injected into nude mice, tumors were obtained. These tumors contain a transfected human rasH gene. Genomic DNA transfection into a line of mouse epithelial cells, in combination with the selection of stable transfectants and tumor induction in nude mice, can be used to screen human tumor DNA for the presence of activated oncogenes.