利用单纯疱疹病毒胸苷嘧啶激酶建立肝脏特异损伤的转基因大鼠模型

目的观察单纯疱疹病毒胸苷嘧啶激酶（HSV—tk）在建立肝脏特异损伤的转丛凶大鼠模刷中的作用。方法选取鼠龄7～8周的雄性Wistar大鼠40只，通过HSV-tk载体进行转基因大鼠雄原核显微注射，获得了目的基因HSV—tk整合与特异表达的转基因大鼠，进一步通过尾静脉注射世泞洛韦（GCV）诱导转基因大鼠肝脏损伤，以四氯化碳（CCl4）损伤大鼠为对照组观察疾病的进程。通过血液的生化检查、肝脏与。肾脏等组织的病理形态学分析来研究转基因大鼠的损伤效应。结果（1）质粒pLLtk比质粒pLLtkcut对HepG2细胞有更高的杀伤效应（32％提高到53％）。（2）F1代tk转基因大鼠除肝脏与睾丸外其他组织与器官均没检测到HSV-tk的转录，说明HSV-tk的表达具有良好的组织特异性。（3）所有F1代tk大鼠在GCV处理后，经过血液生化指标与组织病理形态学检查产生了生理功能与形态学改变的肝脏损伤。（4）tk转基凶大鼠肝脏组织进行病理形态学分析，结果渺爪病理形态学普遍表现为点状或病灶性坏死，炎性细胞浸润，有凋亡细胞存在，肝细胞增生。结论成功研制肝脏表达HSV—tk的转基因大鼠，通过GCV注射诱导肝脏损伤后，产生了具有组织病州形态学与临床生物化学特征的肝细胞疾病模型。

小鼠ALB启动子/增强子驱动HSV-tk对肝脏细胞的杀伤效应(英文)

利用小鼠白蛋白 (ALB)启动子 /增强子及单纯疱疹病毒胸苷嘧啶激酶 (HSV tk)DNA构建了载体pLLTK ,以研究该载体对肝脏细胞的特异性杀伤效应。首先 ,为了比较载体的肝脏细胞特异转录活性 ,以绿色荧光蛋白 (GFP)基因为报告基因构建了载体 pLE (仅含小鼠ALB启动子 )、pLLE(含小鼠ALB启动子和上游增强子 )和 pLEL(含小鼠ALB启动子和下游增强子 ) ,分别转染到人肝细胞株Hep G2与小鼠乳腺上皮细胞株HC 11,荧光显微镜与流式细胞术分析GFP的表达。然后将载体pLLTK转染到Hep G2研究对细胞的杀伤效应。结果发现 :小鼠ALB启动子 /增强子能驱动GFP肝脏特异表达 ;HSV tk在Hep G2表达使细胞具有更昔洛韦 (GCV)敏感性 ,在GCV作用 7d后 ,MTT分析细胞的生存率 ,pLLTK转染细胞表现明显的细胞死亡 (5 3% ) ,而阴性对照组pcDNA3 1转染细胞没有明显变化 (仅 2 %细胞死亡 )。以上结果表明所有的载体具有肝脏细胞特异性 。

^(18)F-FDG和^(18)F-FLT的合成及其应用研究

"一锅法"合成^(18)F-FLT和^(18)F-FDG两种显像剂,并用于食管癌放疗疗效的监测。结果表明:^(18)F-FDG的总合成时间约25 min,未经校正的放化产率约为55%;^(18)F-FLT总合成时间约53 min,未校正放化产率约20%;^(18)F-FLT在鉴别肿瘤和炎性组织时比^(18)F-FDG更具有特异性。

^(18)F-FLT PET/CT与MRI在脑胶质瘤放射治疗靶区勾画中的比较研究

目的通过对脑胶质瘤术后患者在放疗前分别进行MRI、^(18)F-FLT PET/CT显像,探讨在CT图像上分别联合上述两种显像方式进行靶区勾画,观察其对胶质瘤靶区勾画及放疗计划的影响。方法对14例脑胶质瘤术后经MRI检查认为存在术后残留的患者进行^(18)F-FLT PET/CT显像检查,对所有患者分别在增强CT图像与^(18)F-FLT PET/CT或MRI融合显像上进行靶区勾画,之后应用计划系统进行2组影像的靶区比较。结果在MRI和^(18)F-FLT PET/CT上勾画出的靶区体积差异有统计学意义(Z=3.545,P<0.05),GTV和CTV均为PET/CT高于MRI,GTV PET比GTV MR平均增大2.53 cm^(3),CTV PET比CTV MR平均增大6.79 cm^(3)。不同医师之间在MRI及PET/CT上勾画的GTV差异均无统计学意义(χ^(2)=0.143,P>0.05);不同医师在MRI上勾画的GTV与在PET/CT上勾画的GTV最大值与最小值之间差异无统计学意义(Z=0.785,P>0.05),PET/CT组的GTV离散程度为5.69 cm^(3),MRI组GTV离散程度为7.86 cm^(3)。在MRI和PET-CT上勾画GTV、CTV的靶区重合度差异有统计学意义(TC GTV=0.642±0.071,t=33.763,P<0.05;TC CTV=0.709±0.067,t=39.622,P<0.05)。结论以MRI和^(18)F-FLT PET/CT为辅助影像勾画出的靶区体积及重合度存在差异性,二者显示的肿瘤范围不同;不同勾画者在MRI及PET/CT上勾画的GTV及CTV体积无差异性,但PET/CT组的GTV离散度较MRI组小,说明不同医师在^(18)F-FLT PET/CT上勾画的靶区范围认知差异度小。

An Experimental Model for Screening Anti-AIDS Drugs with Bovine Immunodeficiency Virus

The assays for bovine immunodeficiency virus (BIV) induced syncytium formation and BIV long terminal repeat (LTR) directed luciferase (Luc) gene expression were applied to screen and evaluate anti AIDS drugs. Frequency of the syncytium formation and BIV LTR directed Luc activity were in proportion to the number of input BIV infected cells. AZT inhibited the syncytium formation and the BIV LTR directed Luc gene expression level. Its inhibitory effects were dosedependent with the IC 50 being 0.24 and 0.052 mmol / L, respectively.

Research development of the relationship between thymidine phosphorylase expression and colorectal carcinoma

Thymidine phosphorylase (TP) is a key enzyme that contributes to the composition and decomposition of pyrimidine nucleotides. TP seems homologous to platelet-derived endothelial cell growth factor, and its effects on inducing vascularization and anti-apoptosis are closely related to growth and metastasis of colorectal carcinoma. In addition, TP is a key enzyme that catalyzes the transformation from 5-fluorouracil (FU) prodrugs of 5′-deoxy-5-fluorouridine (5′- DFUR) to 5-FU. The activity of TP is closely related to the sensitivity of colorectal carcinoma cells to fluorouracil drugs and targeted therapy. Given the important functions of TP in growth, metastasis, tumor treatment, and prognosis, determining its expression mechanism is significant. This article summarizes the research development of TP expression in colorectal carcinoma, tumor neovascularization, cytotoxicity activation of 5′-DFUR, and colorectal carcinoma therapy.

Retrovirus-mediated herpes simplex virus thymidine kinase gene therapy approach for hepatocellular carcinoma

The therapeutic effect of herpes simplex virus thymidine kinase/ganciclovir (HSV-tk/GCV) system on hepatocellular carcinoma was studied in this experiment. The tk-containing retroviral recombinants were used to infect hepatoma cells (BEL-7402) and the cells were treated with ganciclovir (0-1000 microg/ml). The results showed that HSV-tk gene could be efficiently transferred in vitro into hepatoma cells and stably expressed. The growth potential of the tk-containing cells was significantly inhibited by GCV (P

RNA INTERFERENCE OF ANNEXIN II GENE IN PC3 CELLS BY USING SMALL INTERFERENCE RNA SYNTHESIZED WITH IN VITRO TRANSCRIPTION

Objective To silence annexin Ⅱ gene expression by using small interference RNA （siRNA） in prostate cancer cell line PC3. Methods For in vitro transcription, four sequences of 29-nucleotide DNA template oligonucleotides were designed, and one pair of the sequences were complementary to annexin Ⅱ gene. The other pair was negative control. The 8 nucleotides at the 3＇ end of each oligonucleotide were complementary to the T7 Promoter Primer. The sense and anti-sense siRNA templates were transcribed by T7 RNA polymerase and the resulting RNA transcripts were hybridized to create dsRNA. The siRNA was transfected into prostate cancer cell PC3. For assaying the efficiency of siRNA, confocal microscopy, Northern blotting, and Western blotting were employed to examine the expression of annexin Ⅱ protein and its mRNA. ^3H thymidine was used to measure DNA synthesis. Results The siRNA sequence specific to annexin Ⅱ gene was capable of inhibiting the expression of annexin Ⅱ protein and its mRNA. And cellular DNA synthesis was significantly reduced in siRNA transfected cells.Conclusions The protocol for the synthesis of siRNA by T7 RNA polymerase is feasible. Annexin Ⅱ might be involved in DNA synthesis.

Antitumor effects and radiosensitization of cytosine deaminase and thymidine kinase fusion suicide gene on colorectal carcinoma cells

AIM: To investigate the killing effect and radiosensitization of double suicide gene mediated by adenovirus on colorectal carcinoma cells. METHODS: Colorectal carcinoma cell line SW480 was transfected with adenovirus expression vector containing cytosine deaminase (CD) and thymidine kinase (TK) fusion gene. The expression of CD-TK fusion gene was detected by reverse transcriptase-polymerase chain reaction. The toxic effect of ganciclovir (GCV) and 5-fluorocytosine (5-FC) on infected cells was determined by MTT assay. The radiosensitization of double suicide gene was evaluated by clonogenic assay. RESULTS: After prodrugs were used, the survival rate of colorectal carcinoma cells was markedly decreased. When GCV and 5-FC were used in combination, the cytotoxicity and bystander effect were markedly superior to a single prodrug (X2 = 30.371, P<0.01). Both GCV and 5-FC could sensitize colorectal carcinoma cells to the toxic effect of radiation, and greater radiosensitization was achieved when both prodrug were used in combination. CONCLUSION: CD-TK double suicide gene can kill and radiosensitize colorectal carcinoma cells.

Non-viral targeted delivery system mediates transfection of thymidine kinase gene of herpes simplex virus into ovarian cancer cells:a comparison between one time and continuous mediation

Objective： To compare the transferring efficiency and killing effects of one time and continuous mediation with GE7, a non-viral targeted delivery system, in transfection of thymidine kinase gene of herpes simplex virus （HSV-tk） into ovarian cancer cells. Methods： GE7 was used to prepare recombinants with β-galactosidase （β-gal） and HSVI-tk; the recombinants were then used to transfect human ovarian cancer line CaOV3 once and continuously. β-gal staining was used to compare the efficiencies of one time and continuous mediation with GE7 system. Ganciclovior （GCV） was introduced into HSVI-tk transfected ovarian cells. Through drawing the cell growth curve and flow cytometry, the killing effects of GCV on once and continuously GE7/HSVI-tk transfected cells were observed. Results： We found that the one time and continuous exogenous gene transfer efficiencies were about 80% and 85%, respectively. When 1 μg/mL GCV was used to treat ovarian cell transfected with HSVI-tk gene, growth inhibiting rates of ovarian cells of one time and continuous transferring were 82% and 90%, respectively; their apoptosis indices were 15 and 30, respectively. Under same GCV concentration, continuous mediation of GE7/pCMV-tk transfection into ovarian cancer cells had more significant inhibitory effect than one time mediation （P 〈 0.05）. Conclusion： Compared with one time mediation, continuous mediation of transfection with GE7 gene delivery system has higher efficiency. Continuous mediation of GE7/HSVI-tk/GCV therapeutic gene system has more powerful killing effect.

脑星形细胞瘤术后^(18)F-FLT PET/CT显像中PET参数的诊断意义

目的探讨3′-脱氧-3′-18 F-氟胸腺嘧啶胸苷(3′-deoxy-3′-18 F-fluoro-thymidine,18 F-FLT)分子显像中最大标准摄取值(maximum standardized uptake value,SUVmax)和病灶与对侧正常脑摄取比(L/N),在星形细胞瘤术后复发和放射治疗损伤中的定量分布特点,以利于准确地鉴别诊断。方法 2010-10-01-2013-12-31,对中山大学附属第一医院脑星形细胞瘤术后辅助放疗的29例患者,行18 F-FLT正电子发射及计算机断层显像(positron emission and computer tomography,PET-CT),利用感兴趣区(region of interest,ROI)技术进行定量分析,测定术后放疗病灶的SUVmax和L/N值,对术后复发和放疗损伤2组定量参数进行统计对比分析。结果脑星形细胞瘤术后复发组17例,其中Ⅲ级10例,Ⅳ级7例;平均SUVmax为1.41±0.75,L/N值为3.54±1.05。术后放射治疗损伤组12例,平均SUVmax为0.28±0.06,L/N值为0.82±0.03。上述2组数据的差异有统计学意义,P值均<0.05。结论脑星形细胞瘤术后行18 F-FLT分子显像,其定量参数指标SUVmax和L/N能够提高鉴别术后复发和放射治疗损伤的准确性,对指导临床术后再治疗有重要意义。

三种方法对细胞周期诱导效率的比较

比较两种处理方法对细胞周期调控的影响,本研究用饥饿法,胸腺嘧啶处理法和饥饿法结合胸腺嘧啶法诱导胎儿成纤维细胞进入G1/G0期。诱导两周后,收集3种方法来源的细胞用流式细胞技术、细胞活力检测、real-time PCR和核型分析检查细胞诱导效率、细胞活力、成纤维细胞特异基因的表达水平和核型情况。结果表明,实验组细胞G1/G0期比率显著高于对照组(p<0.05);实验组中,饥饿联合药物诱导法比饥饿法和药物法稍高,但未达显著水准。实验组与对照组细胞核型正常,均为40条染色体,性染色体为XX。细胞活力和显示,对照组比试验组稍高,但差异不显著(p>0.05);FGF4、FGF2及Sox2的基因表达水平在各组间差异不显著(p>0.05)。这些结果表明,实验组3种方法对细胞特性没有显著影响,饥饿结合药物诱导可适当提高细胞诱导效率,为相关研究提供参考。