Retrovirus-mediated transfer of the fusion gene encoding EGFP-BMP_2 in mesenchymal stem cells

Objective To develop retrovirus-mediated transfer of the fusion gene encoding EGFP-BMP_2 in mesenchymal stem cells.Methods Mesenchymal stem cells from New Zealand white rabbits were transduced with retroviral pLEGFP-BMP_2 vector by the optimized retroviral transduction protocol.Fluorescent microscopy's examination was to evaluate the results of the transduction,flow cytometer's analysis was to evaluate the transduction efficiency and the Fluorescence-activated cell sorting method was to sort the transduced cells.Bioactivity test from C_2C_12K_4 cells was to show the expression and bio-activity of the fusion gene.Results Fluorescent microscopy showed the success of the transduction.By flow cytometer's analysis,the mean efficiency of the transduction with EGFP was(42.8±6.1)% SD.Transduced cells were sorted efficiently by the fluorescence-activated cell sorting method and after sorting,almost of those showed the expression of BMP_2.Fluorescently and strongly bioactivity test for C_2C_12K_4 cells demonstrated that fluorescent materials were located the surface of cells and the activity of luciferase increased compared with the control.Analysis of long-term expression showed there was no difference between 2 week-time point and 3 month-time point of culture post-sorting.Conclusion Mesenchymal stem cells can be transduced efficiently by retrovirus-mediated transfer of the fusion gene encoding EGFP-BMP_2,the highly pure transduced cells are obtained by the fluorescence-activated cell sorting technique,the expressed chimeric protein embraced the double bioactivity of EGFP and BMP_2,and moreover,the expression had not attenuated over time.

SEQUENCE STUDY AND RETROVIRUS MEDIATED GENE TRANSFER IN MAMMALIAN CELL SYSTEMS OF HUMAN INTERLEUKIN 2 cDNA

Interleukin 2 (IL- 2) is a T cell growth factor. In the present study, human IL- 2 cDNA was cloned from total RNA of activated tonsillar mononuclear cells (TMNC) following reverse transcription and PCR amplification using a pair of synthesized primers. DNA sequence analysis demonstrated that the IL- 2 cDNA cloned from the Chinese tonsil donor is identical with the data reported so far, reflecting the high structural conservation of this gene. The human IL- 2 cDNA was inserted into XM6 to construct a recombinant retroviral expression vector XM6-IL2, having human IL-2 cDNA driven by the 5' LTR of MMLV. This vector was successfully passaged through ψ 2 and PA317 cells to yield high producer lines of ecotropic and amphotroplc infectious viruses. The murine myeloma cell line SP2/0 after being infected by retrovirus released from high titer PA317 constitutlvely secreted IL- 2 activity into the culture medium when assayed for T cell proliferative capacity. Activated human T cells are also exposed to the infectious retrovirus XM6- IL2. In sharp contrast to the parallel controls, the infected T cells with or without the furtheraddition of 500 units/ ml of exogenous IL- 2 proliferated and formed colonies of significant size under the selection pressure of G418. However, their growth in vitro could only be maintained for about 3 weeks. These facts demonstrated that gene transfer of human IL- 2 cDNA viaretrovirus is far from being sufficient to maintain the relatively long-termgrowth and clonal expansion of human T cell subpopulations in vitro.

CONSTRUCTION AND EXPRESSION OF ADENO-ASSOCIATED VIRUS-BASED PLASMID EXPRESSING VECTORS CONTAINING hIL-2 GENE OR mIFN-γ GENE

Obiective TO improve the plasmid vectors in gene therapy, adeno - associated virus (AAV) basedplasmid expressing vectors containing hIL - 2 gene or mIFN-γ gene were constructed and its expression intransfected cells was studied. Methods By means of step to step cloning, promoter CMVp was placed at thedownstream of 5’ inverted terminal repeat from AAV (AAV - ITR) of pAP, hIL - 2 gene or mIFN -γ gene insertedinto pAC between CMVp and polyA. Then intron A was inserted into pAC - hIL - 2 or pAC- mIFN-γ betweenCMVp and IL - 2 gene or IFNγ gene to construct pAI- hIL - 2 or pAI- mIFN -γ. Liposome - plasmid complexeswere formed by mixing Dosper with these AAV- based plasmids containing hIL - 2 gene or mIFN- γgene. Results High biotogical activities of IL - 2 or IFN- γ could be detected in the supernatants of NIH3T3 andMM45T Li cells after transfection. Insertion of intron A into pAC- hIL - 2 or pAC- mIFN - γ improved theexpression of IL - 2 or IFN- γ. Conclusion These data demonstrated that the constructed AAV-based plasmidexpressing vectors could ejlciently express therapeutic genes in cultured cells and could be used as a nonviral genetransfer system in human gene therapy.

逆转录病毒载体介导IL-2基因转染人肝细胞的建立及其部分生物学性状

目的 建立ｈＩＬ－２基因修饰的人肝细胞株并探讨对其生物学活性的影响。 方法应用重组逆转录病毒载体ｐＬＮＣＩＬ－２，将ｈＩＬ－２基因导入人肝细胞系Ｌ－０２，观察其形态及克隆形成率的变化，检测细胞培养上清中ｈＩＬ－２的含量，以及进行转染细胞基因组ＤＮＡ ＮｅｏＲ基因片段的ＰＣＲ扩增。结果Ｌ－０２／ＩＬ－２细胞的增殖速度和克隆形成率低于Ｌ－０２／Ｎｅｏ细胞和Ｌ－０２细胞。Ｌ－０２／ＩＬ－２细胞的培养液中ｈＩＬ－２的含量达３２ ０００ ｐｇ／１０６ｃｅｌｌｓ·ｄ，并可持续表达１０ ｗｋ以上。从Ｌ－０２／ＩＬ－２细胞和Ｌ－０２／Ｎｅｏ细胞基因组ＤＮＡ中，均扩增到ＮｅｏＲ基因片段（７９０ ｂｐ）。结论应用重组逆转录病毒载体成功地建立了Ｌ－０２／ＩＬ－２细胞株，为进一步进行肝细胞移植动物实验奠定了基础。

逆转录病毒介导IL-2基因转移对K562细胞增殖周期的影响

应用逆转录病毒载体将IL-2基因导入人红白血病细胞系K562细胞中。转导18天后,细胞DNA周期分析发现空载体转导的细胞K562/neo及含IL-2基因载体转导的细胞k562/IL-2的G0/G1期比例降低,而G2+M期增高。转导30天后K562/neo DNA周期分布恢复至转导前水平,而K562/IL-2细胞G0/G1期比例仍低于未转导细胞,G2+M期仍高于未转导细胞。MTT法检测细胞增殖活性观察到K562/IL-2从培养第4天起增殖活性明显落后于未转导细胞,核分裂指数亦低于水转导细胞。光学显微镜观察见K562/IL-2细胞中出现较多巨大细胞及多核巨细胞,细胞核数目可多达20余个,推测多核巨细胞的形成可能与细胞核反复分裂而胞质不能分裂有关。进一步形态计量学分析证实IL-2基因修饰的K562细胞体积增大,巨大细胞出现率显著高于未转导的K562细胞。结果提示K562/IL-2细胞体积增大与G2+M期细胞比例增高有关,推测IL-2基因修饰可能导致K562细胞周期滞留于G2期。

IL-2、IL-4基因转染后肿瘤细胞表面ICAM-1分子的表达及其作用

为了进一步研究细胞因子基因转染后肿瘤细胞体内致癌原性、免疫原性变化的分子 机制，将ＩＬ－２、ＩＬ－４ 基因转染入Ｂ１６黑色素瘤细胞，观察了其体内接种后致瘤原性变化，通过 ＦＡＣＳ法检测了其细胞表面粘附分子－１（ＩＣＡＭ－１）的表达水平，分析了其细胞表面 ＩＣＡＭ－１表达水 平以及它们与肿瘤细胞对ＬＡＫ、ＣＴＬ等免疫效应细胞杀伤敏感性变化的关系。结果表明，ＩＬ－２、ＩＬ－ ４基因转染后Ｂ１６细胞体内致瘤原性明显降低，其细胞表面ＩＣＡＭ－１的表达高于野生型Ｂ１６细胞， 且对ＬＡＫ、ＣＴＬ细胞的杀伤敏感性增加。抗ＩＣＡＭ－１单抗可以阻断ＩＬ－２、ＩＬ－４基因转染后Ｂ１６细 胞对ＬＡＫ、ＣＴＬ杀伤敏感性的增强效应。表明细胞因子基因转染后Ｂ１６细胞体内致瘤原性改变除 与其诱导或增强机体的抗肿瘤免疫反应有关外，还与细胞表面ＩＣＡＭ－１分子的表达增加从而使其 对免疫效应细胞的杀伤敏感性增强有关。

联合应用hIL-2和hGM-CSF基因瘤苗抗肿瘤作用的研究

目的 :探讨联合应用人白细胞介素 2 (hIL 2 )和人粒细胞巨噬细胞刺激因子 (hGM CSF)基因瘤苗抗肿瘤作用。方法 :经逆转录病毒载体将hIL 2基因及hGM CSF基因导入大鼠Walker瘤细胞WRC2 5 6中 ,制备瘤苗接种荷瘤大鼠。结果 :经PCR SouthernBlot检测证实hIL 2基因及hGM CSF基因已成功导入WRC2 5 6细胞基因组中 ,经生物学活性检测证实转基因细胞具有分泌hIL 2及hGM CSF活性。转基因瘤苗经 6 0GyX线灭活 ,接种荷瘤Walker瘤模型。两种瘤苗确可诱导有效抗肿瘤反应 ,但与单独应用一种瘤苗相比较 ,联合应用无相加或协同作用。结论 :两种瘤苗可诱导有效抗肿瘤反应 。

腺病毒介导hIL-2基因转染膀胱上皮的体内研究

目的:探讨腺病毒介导人IL-2基因转染鼠膀胱移行上皮细胞及其表达的可行性,为膀胱癌的免疫治疗提供实验依据。方法:通过膀胱灌注的方法将重组腺病毒AdhIL-2灌入大鼠膀胱内,分不同时间段获取大鼠膀胱黏膜组织,利用RT-PCR的方法检测hIL-2基因在膀胱移行上皮细胞中的表达。结果:腺病毒介导hIL-2在膀胱移行上皮细胞中得到有效表达,基因表达持续时间达到7天。结论:腺病毒是一种有效介导基因的工具,hIL-2在膀胱上皮细胞中的持续表达为膀胱癌免疫治疗提供新的方法。

IL-2基因转移对卵巢癌细胞系SKOV3细胞周期及TGF-β_1表达的影响

目的 探讨人白细胞介素2(IL-2)基因转移对卵巢癌细胞周期和转移生长因子β_1(TGF-β_1)表达的影响。方法 采用流式细胞术探讨IL-2基因转移对卵巢癌细胞SKOV3细胞周期及TGF-β_1表达的影响。结果 SKOV3/IL-2细胞GO、G1期细胞比例明显高于对照组,而S、M期细胞明显少于对照组,P<0.001,表现为G0/G1期阻滞。SKOV3、SKOV3/Neo、SKOV3/IL-2细胞TGF-β_1阳性百分率及荧光强度分别为98.64％、97.00％、99.52％和143、138、163,SKOV3/IL-2平均荧光强度较亲本细胞明显提高,P<0.001,差别非常显著。结论 IL-2基因转移可引起卵巢癌细胞系SKOV3细胞周期G0/G1期阻滞,TGF-β_1表达的增强有可能是IL-2基因转移诱发细胞增殖抑制的原因之一。

IL-2基因转导对卵巢癌细胞化疗药物敏感性的影响

目的:探讨IL-2基因转导能否改变卵巢癌细胞对化疗药物的敏感性。方法:用MTT法测定导入人IL-2基因的卵巢癌细胞对化学治疗药物顺铂、阿霉素、泰素及足叶乙甙治疗的敏感性及IC_50,以导入新霉素基因的卵巢癌细胞系及野生型卵巢癌细胞系为对照。结果:IL-2基因转移使SKOV3细胞对上述化疗药物治疗的敏感性有所提高,但仅对VP-16治疗敏感性的提高差异有显著性（P<0.05）。结论:IL-2基因导入SKOV3细胞没有降低其对实验药物治疗的敏感性。

以逆转录病毒为载体的IL-2基因转染K562细胞的研究

目的 :研究以逆转录病毒为载体将IL 2基因转入K5 62细胞及表达情况。方法 :应用脂质体介导的基因转移法 ,将质粒PGEN/IL 2导入包装细胞PA317,将K5 62细胞与PA317/IL 2细胞共培养 ,检测IL 2cDNA整合 ,mRNA转录情况 ,以IL 2依赖性CTLL 2细胞测定培养细胞上清中IL 2产量 ,比较转染前后细胞的体外生长情况和致瘤性。结果 :IL 2cDNA成功整合入K5 62细胞基因组中并稳定表达 ,K5 62 /IL 2细胞培养 2 4h上清中IL 2活性为 10 0U/ml,体内外观察均见细胞生长减慢。结论 :以脂质体介导的以双顺反子逆转录病毒为载体的基因转移方法 ,可成功地将人IL 2基因转入人白血病细胞株K5 62 ,并持续分泌高活性的IL 2 ,为下一步将IL 2基因转入CML造血细胞的研究打下基础。

腺病毒介导人白介素-10转基因对大鼠同种异体移植血管IL-2、TNF-α的影响

目的:观察腺病毒介导人白介素-10(hIL-10)转基因对大鼠同种异体移植血管IL-2、TNF-α的影响及其可能的作用机制。方法:以Wistar大鼠为供体,SD为受体,采用颈动脉显微外科原位吻合技术,将经直接浸泡法转染腺病毒介导hIL-10的离体供血管植入受体血管。随机分为3组:I组(空白对照组,n=9),II组(空载体组,n=10),III组(基因转染组,n=10)。移植后5d,观察移植物病理组织学变化及免疫排斥级别;RT-PCR、ELISA、免疫组化染色检测移植血管hIL-10基因产物;免疫组化染色检测IL-2、TNF-α。结果:基因转染组移植血管有效地表达特异性hIL-10基因产物。与对照组比较,急性排斥级别降低(P<0.01);IL-2、TNF-α的表达量明显下降(P<0.01)。结论:腺病毒介导人白介素-10转基因能有效地下调IL-2、TNF-α表达,诱导移植血管局部免疫抑制状态,抑制同种异体移植血管的急性排斥反应。

IL-2基因转导CD_3AK细胞免疫学功能的研究

目的 :观察白细胞介素 2 (IL 2 )基因转导后CD3AK细胞免疫学功能的变化。方法 :应用逆转录病毒载体将IL 2基因转导入CD3AK细胞。检测转导细胞中特异性NeoR 基因、培养上清IL 2的表达水平及转导CD3AK细胞的体外增殖活性、细胞毒活性和细胞表型。结果 :从转导细胞mRNA中扩增出长度为 347bp的特异性NeoR 基因片段 ,转导细胞培养上清的IL 2表达水平显著增高 ,体外增殖活性和细胞毒活性均强于未转导组细胞 ,CD4 +/CD8+值升高。结论 :PLIL 2SN逆转录病毒转导CD3AK细胞后 ,IL

K562细胞导入IL-2基因后的细胞凋亡

应用逆转录病毒载体介导人白细胞介素2(IL-2)基因转入人红白血病细胞系K562并获得表达。IL-2基因修饰的细胞发生了明显的形态学改变,胞质空泡化,胞浆嗜碱性减弱,核出现分叶现象,同时可见部分细胞核染色质凝集于核内膜处,核膜完整,细胞器保存完好,并可见细胞的发疱现象,提示IL-2基因转导可诱导K562细胞凋亡。

逆转录病毒载体PLIL-2SN转导人CD_3AK细胞方法的建立

目的 :探讨CD3AK细胞在基因治疗中的应用 ,并对逆转录病毒载体转导CD3AK细胞IL 2基因的方法进行研究。方法 :利用逆转录病毒载体PLIL 2SN向人CD3AK细胞中导入IL 2基因。结果 :从转导细胞中RT PCR扩增出 347bpNeoR 基因特异性片段 ,并测出培养上清液中IL 2浓度为 3 .2 76 μg·L-1。结论 :转导的IL 2基因得到表达 ,转导成功。这有助于进一步研究转导后淋巴细胞的功能 。

The Experimental Study on Treating Transgenic HBV Mice with Recombined IL-2-PreS DNA Vaccine

The aim of this study is to investigate the feasibility and mechanism of hIL-2-preS DNA vaccine as prevention and therapeutic approach against Hepatitis B. Eukaryon expression vector involving hIL-2 and preS gene was constructed with recombinant technique and transferred into normal BALB/c mice and HBV transgenic mice (Tg-Mice) respectively. Then a series of detection were performed: detection of anti-preS2, HBs antibody and HBsAg in BALB/c mice and Tg-mice with ELISA, quantification of HBV DNA copies in HBV Tg-mice serum with real-time PCR, determination of hepatitis degree with immunopathological HE staining and detection of liver function. Anti-preS1 can be detected at 4 th , 6 th and 10 th week in inoculated BALB/c mice. Injection with gene gun gained an advantage over muscular and subcutaneous injection since it acquired just 1/10 inoculation quantity (10 μg/mouse). Highest expression of IgG2a at 4 th week suggested Th1-mediated immune response, which facilitated HBV cleaning. Of all inoculated HBV Tg-mice, 80% of them showed anti-preS2, HBs antibody positive and HBV DNA decreased, and 20% showed negative for HBsAg. HE staining to hepatic tissue showed obvious infiltration of inflammatory cells, swelling and granular degeneration of hepatocytes. In our study, IL-2-preS DNA vaccine which can provoke the humoral and cellular immune response and break the immune tolerance supports the designation and construction of new vaccine against HBV and specific immune remedy for HBV continuous infection.

人白细胞介素2重组逆转录病毒载体的构建与表达

通过RT-PCR克隆到含有全部编码序列的人IL-2 cDNA．并经核苷酸测序加以证实，将其克隆至逆转录病毒载体pLXSN，构建成人IL-2的重组逆转录病毒表达载体pLXSN-hIL2．体外经CRIP细胞包装后病毒滴度达7.6×10^4CFU／ml,NIH 3T3小鼠成纤维细胞感染hIL-2重组逆转录病毒后．分泌IL-2水平达118.2U／ml；PCR从其基因组DNA中扩增到NeoR基因片段．提示重组逆转录病毒载体已整合至宿主细胞的基因组DNA中。本研究为开展人IL-2基因治疗奠定了基础.

白细胞介素2基因转移的肿瘤细胞克隆的建立及其体内外生长特性的研究

为了开展ＩＬ－２基因转移后免疫原性增强的新型瘤苗抗肿瘤作用的研究，须首先获得ＩＬ－２基因转移后、能够高分泌ＩＬ－２的肿瘤细胞并确定其生长特性。本室构建了含５６３ｂｐ的小鼠ＩＬ－２全长ｃＤＮＡ的真核表达载体ＢＭＧＮｅｏ－ＩＬ－２，采用磷酸钙ＤＮＡ共沉淀法将ＢＭＧＮｅｏ－ＩＬ－２转移入Ｂ１６黑色素瘤细胞中，通过Ｇ４１８抗性筛选、有限稀释法及活性检测，获得一株高分泌ＩＬ－２（５０６Ｕ／ｍｌ）克隆，并经Ｓｏｕｔｈｅｒｎ印迹法证实ＩＬ－２基因已转入该克隆中。结果表明ＩＬ－２基因转移的肿瘤细胞体外生长能力没有明显变化，但体内致瘤原性显著下降，从而为制备新型瘤苗打下了基础。

骨形成蛋白2基因修饰的骨髓基质细胞与纤维蛋白复合物修复兔关节软骨缺损

目的研究骨形成蛋白2(bone mophogenetic protein 2, BMP-2)重组腺病毒(adenovirus)转染骨髓基质细胞(mesenchymal stem cells, MSCs)后,与纤维蛋白凝胶构成的复合物(Ad-BMP-2+MSCs-纤维蛋白凝胶)对兔关节软骨缺损修复的影响. 方法①Ad-BMP-2转染原代培养的MSCs,通过RT-PCR、细胞免疫组织化学染色、甲苯胺蓝染色等观察转染后3～9 d的MSCs其BMP-2、Ⅱ型胶原及蛋白多糖转录、表达水平的变化.②转染后的MSCs种植于纤维蛋白凝胶,在体外培养1～9 d,通过上述指标及透射电镜观察三维培养条件下其软骨基质的产生.③42只日本大耳白兔先制成直径4.5 mm全层软骨缺损模型,随机分为3组(n=14):A组为Ad-BMP-2+MSCs-纤维蛋白凝胶修复组,B组为MSCs-纤维蛋白凝胶修复组,C组为空白对照组.术后4、8和12周取材行大体观察、HE染色、甲苯胺蓝染色、Ⅱ型胶原免疫组织化学及12周关节软骨弹性常数检测. 结果①Ad-BMP-2转基因MSCs的BMP-2、Ⅱ型胶原 mRNA RT-PCR检测分别在3、5 d呈阳性,与对照组比较差异有统计学意义(P<0.05).②转基因MSCs三维培养物免疫组织化学和甲苯胺蓝染色呈阳性,电镜显示细胞生长良好,有基质合成.③A组各时间点大体、组织形态学和组织化学染色均显著优于B组和C组,12周时力学和组织学已接近正常关节软骨. 结论 Ad-BMP-2能通过促进MSCs分泌BMP-2,诱导Ⅱ型胶原和蛋白多糖的表达,在纤维蛋白三维支架中形成软骨基质,移植入兔关节软骨缺损区可修复直径4.5 mm缺损,其修复组织成分接近正常软骨.

逆转录病毒转染法建立兔VX-2多药耐药株

目的 :建立VX 2多药耐药 (MDR )细胞 (VX 2mdr1 ) .方法 :利用逆转录病毒转染法将带有mdr1cDNA全序列的逆转录病毒载体 pHaMDR1转入到兔VX 2细胞中 ,MTT法检测细胞在不同化疗药物作用下的存活率 ;免疫组化检测细胞的P 糖蛋白 (P gp)表达 ,RT PCR检测细胞内mdr1mRNA的表达量 .结果 :转基因的细胞对吡柔比星、秋水仙素的耐药性分别提高 1 0和 2 5倍 ,免疫组化见转基因细胞中P gp表达增加 ,RT PCR示细胞内mdr1mRNA的表达量增加 .结论 :利用逆转录病毒转染法构建了兔VX