Immunological Adjuvant Function of Aluminium Phosphate and Chicken IL-18 in NDV F Gene Vaccine

[Objective] This study aimed to investigate the immunological adjuvant function of aluminium phosphate and chicken IL-18 in NDV F gene vaccine. [Method] The vaccine （0.2 ml） containing aluminum phosphate adjuvant （90 μg）, pcDNA/F （200μg）, and pcDNA/chlL-18 （200 μg） was prepared. The 7 d old chick- ens to be tested were randomly divided into six groups （12 chickens in each group） and immunized through intramuscular injection with inactivated Newcastle disease vaccines, pcDNA/F＋pcDNA/chlL-18＋phosphate aluminum, pcDNA/F, pcDNA/F.＋pcDNA/ chlL-18, pcDNA/F＋aluminum phosphate, and physiological saline respectively; the secondary immunization was conducted with the same dose when the chickens were 21 d old. Their blood was sampled 0, 7, 14, 21, 28 d after first immunization. Anti- body titer was detected with ELISA and T cell transformation rate was measured with MIT. Experimental chicken will be challenged with 30 LD50 NDV virulence 28 d after first immunization. [Result] The survival rate of the chickens immunized with pcDNA/F＋aluminium phosphate＋pcDNA/chlL-18 achieved 8/12, higher than that of those immunized with pcDNA/F 4/12 and pcDNA/F＋pcDNA/chlL-18 （6/12）. The NDV antibody titer of the chickens immunized with pcDNA/F＋ aluminum phosphate, pcD- NA/F＋pcDNA/chlL-18 and pcDNA/F＋pcDNA/chlL-18＋aluminum phosphate is not differ- ent （P〉0.05）, but significantly lower than that of the chickens immunized with tradi- tional vaccine （P〈0.05）. The T cell transformation rate of the chickens immunized with pcDNA/F＋pcDNA/chlL-18＋aluminium phosphate was obviously higher than that of the chickens immunized with pcDNA/F （P〈0.05）. The T cell transformation rates of chickens immunized with pcDNA/F and the traditional vaccine showed no signifi- cant difference （P〉0.05）. [Conclusion] Combination of aluminium phosphate and pcD- NA/chlL-18 can significantly enhance the immune effect of NDV F gene vaccine.

THE BIOLOGICAL CHARACTERISTICS OF ADENOVIRUS-MEDIATED IL-18 GENE-MODIFIED MURINE COLORECTAL ADENOCARCINOMA CELL IN VIVO AND IN VITRO

Objective: Interleukin 18 (IL-18) is a strong activator of NK cells and promotes the generation of IL-2, IFN-γ and GM-CSF. In the present study, we constructed adenovirus encoding IL-18 gene (AdIL-18), and observed the biological characteristics of IL-18 gene-modified murine colorectal adenocarcinoma cell (CT26)in vivo andin vitro. Methods: Gene modification was mediated by adenovirus. The proliferation of the cells was determined by MTT and IL-18 was assayed by ELISA. The cytotoxicity of NK and CTL was detected by four-hour51Cr release assay. Results: IL-18 gene modification had no effect on the proliferation and morphology of CT-26 cellsin vitro, but the growth of IL-18-modified CT26 cells was obviously inhibitedin vivo. In addition, although IL-18-modified CT26 cells could form tumor nodulesin vivo as well as LacZ-modified CT26 cells or wild-type CT26 cells, the mean survival time of the mice inoculated with IL-18-modified CT26 cells was significantly prolonged as compared with that of control groups. Thus, the anti-tumor immune responses were induced in the group of mice inoculated with IL-18-modified CT26 cells, which might be related to the activation of NK cells and CTL. However, all the three groups ultimately died of tumor. Conclusion: IL-18-modified CT26 cells could induce the anti-tumor immune responses incompletely, which required other factors for effective anti-tumor responses.

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。

IL-18基因转染膀胱癌细胞的建立及其抑瘤作用研究

目的将IL-18基因转染膀胱癌细胞(T24),检测该细胞体内外的凋亡变化,探讨IL-18的抗肿瘤作用机制。方法用含IL-18的基因IL-18/PA317转染T24细胞,经G418筛选后获得IL-18/T24阳性克隆。采用RT-PCR鉴定转染细胞mRNA的表达;用ELISA法检测IL-23/MA-891细胞培养上清中IL-18的分泌;用MTT比色法检测细胞体外增殖能力;观察IL-18/T24细胞生长情况、移植瘤的生长情况;用流式细胞技术检测体外和体内的细胞凋亡率。结果成功将IL-18基因转染T24细胞获得高表达IL-18细胞IL-18/T24。转染IL-18基因不影响T24细胞的体外生长和细胞凋亡,但体内IL-18基因转染组肿瘤生长明显受到抑制,肿瘤组织细胞凋亡率增高(P<0.01)。结论转染IL-18基因后对膀胱癌细胞(IL-18/T24)的体外凋亡无影响,但在体内IL-18能够诱导细胞凋亡,产生抗明显肿瘤作用。

H5亚型AIV HA1基因与鸡IL-18基因共表达载体的构建及其表达

参考GenBank上发表的H5亚型禽流感(AIV)血凝素(HA)基因序列及鸡白细胞介素18成熟蛋白(mChIL-18)的cDNA基因序列,分别设计了HA1和mChIL-18基因的2对引物。然后分别以pMD18-T-HA质粒和pGEX-mChIL-18质粒为模板,扩增出了H5亚型AIV的HA1基因和mChIL-18的cDNA片段。再以杆状病毒pFast-BacTMdual为载体,将H5亚型AIV HA中的HA1基因和mChIL-18基因分别插入到双表达载体pFastBacTMdu-al的p10启动子(PP10)和多角体蛋白启动子(PPH)的下游,构建携带HA1基因和mChIL-18基因的重组pFastBacTMdual-HA1-mChIL-18真核表达质粒。最后将构建的真核表达质粒转座入大肠杆菌DH10Bac,并利用昆虫细胞进行转染。这个重组载体的构建为考察mChIL-18作为免疫增强剂的作用及下一步AIV疫苗的研究奠定了坚实的基础。

pSecTag2B-mIL-18真核分泌表达载体的构建及其抗肿瘤作用研究

目的:探索小鼠IL-18基因治疗肿瘤的方法和疗效。方法:构建pSecTag2B-mIL-18真核分泌表达载体,并用其转染HT-29细胞,RT-PCR和ELISA检测IL-18表达情况;将转染pSecTag2B-mIL-18质粒的HT-29培养上清,加入到小鼠T淋巴细胞培养液,ELISA、RT-PCR检测T淋巴细胞分泌IFN-γ;脂质体包被的pSecTag2B-mIL-18裸质粒,采用肌肉注射法转入Balb/c小鼠,检测IL-18蛋白表达情况;在Balb/c小鼠接种小鼠co-lon-26肿瘤细胞的同时,将表达载体pSecTag2B-mIL-18转入,观察抑制肿瘤生长的情况。结果:1)经酶切和测序鉴定,pSecTag2B-mIL-18真核分泌表达载体所表达的基因序列经比对完全正确。2)pSecTag2B-mIL-18转染HT-29细胞后,IL-18在mRNA和蛋白水平高表达。3)转染后的HT-29培养上清可刺激小鼠T淋巴细胞高水平分泌IFN-γ。4)用裸质粒肌肉注射法将pSecTag2B-mIL-18转入Balb/c小鼠,证明质粒均能够在小鼠肌肉中表达,且表达的蛋白均能分泌到外周血液循环中。5)接种co-lon26细胞的Balb/c小鼠,将pSecTag2B-mIL-18转入小鼠,结果表明IL-18单独应用能明显抑制肿瘤的生长。结论:pSecTag2B-mIL-18裸质粒肌肉注射具有显著的抗肿瘤作用。

外源性IL-18基因对C6胶质瘤细胞增殖及相关基因表达的影响

目的:研究IL-18基因转染对C6胶质瘤细胞增殖活性及相关基因表达的影响.方法:用流式细胞仪观察C6/IL-18细胞周期、增殖指数的变化;用RT-PCR,蛋白印迹、免疫细胞化学方法分析C6/IL-18细胞cyc lin D1,cyc lin B1,Bc l-2 mR-NA及蛋白的表达.结果:与亲代C6细胞相比,C6/IL-18细胞表现为G0/G1期细胞增多、G2/M期细胞减少,细胞增殖指数(PI)降低.C6/IL-18细胞的cyc lin D1和cyc lin B1,Bc l-2 mR-NA及蛋白表达降低.结论:外源性IL-18基因可降低C6细胞的增殖活性,其机制可能与Bcl-2,cyclin B1和cyclin D1表达下调有关.

IL-18基因转染对小鼠卵巢癌OVHM细胞体内成瘤的影响

目的分析转染IL-18基因后,对小鼠卵巢癌OVHM细胞体内成瘤的影响,初步探讨IL-18基因转染治疗卵巢癌的应用价值。方法将逆转录病毒携带的小鼠IL-18基因成功转染至OVHM(OVHM/IL-18),以空载体转染的OVHM(OVHM/LXSN)和野生型(OVHM)作为对照,于裸鼠皮下分别接种细胞,观察各组种植瘤生长情况,计算成瘤率;HE染色及电镜分别观察病理组织切片的形态学改变。结果三组裸鼠的成瘤率相同,但OVHM/IL-18组成瘤时间较晚,随瘤龄增长肿瘤生长缓慢;瘤组织较小、界限清楚,血供不丰富,瘤细胞数量少、恶性程度较低,可见中性粒细胞、淋巴细胞浸润及细胞凋亡、组织坏死现象。OVHM组和OVHM/LXSN组的瘤组织较大、与周围组织界限不清,血管丰富,瘤细胞密集、恶性程度较高。结论IL-18基因成功转染后,可能通过促进肿瘤细胞凋亡、抑制肿瘤血管形成及促进免疫浸润等机制,达到抑制肿瘤生长、降低卵巢癌恶性程度的抗瘤作用。

IL-18基因转染对大鼠胶质瘤体内生长及肿瘤细胞凋亡的影响

目的分析转染外源性IL-18基因后9L胶质瘤细胞体内成瘤及对肿瘤细胞凋亡的影响。方法用立体定向技术将体外用逆转录病毒转染IL-18基因的9L胶质瘤细胞(9L/IL-18)、转染空载体的9L胶质瘤细胞(9L/LXSN)及未转染的9L细胞接种到F344大鼠颅内建立实验动物模型,观察各组细胞对大鼠的致瘤性,计算成瘤率;原位末端标记法(TUNEL法)检测肿瘤组织中肿瘤细胞凋亡情况,计算各组肿瘤细胞的凋亡率;RT-PCR和Westen Blot法检测肿瘤组织中Bax和Bcl-2的表达。结果三组大鼠成瘤率均为100%;TUNEL法检测结果显示,接种9L/IL-18细胞组肿瘤组织内出现大量凋亡细胞,凋亡率为(22.2±1.02)%,明显高于接种9L/LXSN[(5.7±0.32)%]及9L[(6.4±0.51)%]细胞组(P<0.05);接种9L/IL-18细胞组肿瘤组织中Bax的表达较其他两组升高,Bcl-2的表达较其他两组降低。结论 9L胶质瘤细胞转染外源性IL-18基因后,可通过上调Bax的表达,下调Bcl-2的表达促进肿瘤细胞凋亡,发挥抗肿瘤作用。

IL-18基因转染对小鼠卵巢癌OVHM体外增殖及体内成瘤的影响

目的:分析转染IL-18基因后,对小鼠卵巢癌OVHM细胞体外增殖、凋亡及体内成瘤的影响,初步探讨IL-18基因转染治疗卵巢癌的应用价值。方法:将逆转录病毒携带的小鼠IL-18基因成功转染至OVHM(OVHM/IL-18),以空载体转染的OVHM(OVHM/LXSN)和野生型(OVHM)作为对照。分别采用MTT、FCM检测体外培养细胞的增殖、凋亡及周期分布。于裸鼠皮下分别接种细胞,观察各组种植瘤生长情况,计算成瘤率;RT-PCR检测瘤组织中IL-18mRNA表达;FCM和电镜分析肿瘤细胞增殖、凋亡状况。结果:3组细胞的体外增殖未见明显差异,均无明显凋亡现象,增殖指数、细胞周期分布均无明显差异(均P>0.05)。接种后,3组裸鼠的成瘤率相同,但OVHM/IL-18组成瘤时间较晚,随瘤龄增长肿瘤生长缓慢,瘤组织中IL-18 mRNA阳性表达。OVHM/IL-18组裸鼠种植瘤细胞可见典型的凋亡现象,G0/G1期细胞明显增多,S期细胞明显减少,增殖指数明显降低,凋亡指数明显增高(P<0.01)。结论:IL-18基因成功转染后,虽对体外卵巢癌细胞无直接毒性,但可能在体内借助非直接杀伤的其他途径,通过阻断细胞周期、促进肿瘤细胞凋亡等抑制体内成瘤。

Synthesis of Codon-optimized Human Interleukin-18 Gene by Combination of Chemical and Enzymatic Method

According to the amino acid sequence and codon preference of E. coli, the human interleukin-18（IL-18） gene was optimized to avoid the rare codons. The total length of the synthesized gene is 571 bp; 18 oligonucleotides, DNA fragments were designed and synthesized by the phosphoramidite four-step chemical method. The whole DNA sequence was synthesized by a one-step total gene synthesis method, and then inserted in pUC18 vector. Five positive clones identified by blue-white colony screening were sent to Shanghai Sangon Biological Engineering Technology and Service Co., Ltd. for sequencing. The sequencing result shows that one clone contained the complete correct gene in all the five positive clones.

白细胞介素18基因修饰的树突状细胞的表型分析及其免疫刺激活性

目的:研究IL-18基因修饰后的树突状细胞(DC)的表型和功能的变化.方法:以含IL-18基因的重组腺病毒体外转染小鼠骨髓来源的DC,RLIDS检测IL-18分泌水平,以RT-PCR检测IL-18mRNA表达,以FACS法分析其DC表型变化,采用TdR检测其MLR的变化.结果:IL-18基因修饰的DC有效分泌IL-18,可检测到IL-18mnRNA的表达,分泌上清具有诱导T细胞产生IFN-γ的作用,IL-18基因修饰的DC同种异体MLR明显增强,且仅能被IL-18抗体部分阻断,表型分析表明,IL-18基因修饰后的Ia,B7.2,ICAM-1太阳性的DC的比例明显增加.结论:IL-18基因修饰的DC可有效表达有功能的IL-18,部分表面分子表达上调,刺激同种异体T淋巴细胞增殖能力的提高,提示其抗原提星功能增强.

猪白细胞介素18全基因的克隆、真核表达质粒的构建及其在猪肾细胞中的表达

通过RT-PCR方法自猪脾脏淋巴细胞中扩增mpIL-18基因,序列测定表明,plL-18全基因核苷酸长度为579bp,编码192个氨基酸。将其克隆到真核表达载体pcDNA3.1中,构建重组质粒pcDNA-ILl8m,所获重组质粒经过酶切、测序鉴定,证实含有目的片段,且连接、构建正确。阳性克隆鉴定后,在脂质体作用下转染猪肾细胞(PK15),通过提取RNA检测到了mpIL-18在PK15细胞中的表达。

pIRES2-HPV18E2-EGFP质粒重组及其在HeLa细胞中的表达

目的构建人乳头瘤病毒18型E2基因片段(HPV18E2)重组表达质粒并予以表达,为进一步研制HPV18相关疾病提供材料。方法以重组质粒(pBR322-HPV18)为模板,PCR方法扩增HPV18E2DNA片段,将HPV18E2DNA与加强绿色荧光质粒(pIRES2-EGFP)重组构建重组质粒(pIRES2-HPV18E2-EGFP)。用酶切电泳及测序检查质粒重组后序列正确性。重组质粒转染Hela细胞。RT-PCR鉴定转染细胞中E2基因。结果PCR扩增DNA片段约为1 kb,与预期结果相同。克隆重组质粒pIRES2-HPV18E2-EGFP酶切后显示的酶切图谱与预期相同,而且测序验证插入片段全序列无改变。转染并用G418筛选后,在荧光显微镜下可见绿色荧光细胞的表达。转染细胞RT-PCR出现特异性条带。结论成功构建表达HPV18 E2蛋白的靶细胞模型。

Analysis Tissue Expression of IFN-γin IL-12 and/or IL-18 Gene Ablated Na(?)ve Mice

Interleukin 12(IL-12)and/or interleukin 18(IL-18)gene ablated mice were applied for the investigation of the tissue expression of interferon γ(IFN-γ).For IL-12^(-/-),IL-18^(-/-),IL-12^(-/-)/18^(-/-) and wt mice,reproductive performance were recorded and IFN-γ concentrations in heart,lung,liver,spleen,kidney and serum were quantified by ELISA. There were no significant differences of IFN-γ in heart,lung and kidney between 4 strains although control group was higher.It was observed that for IL-12^(-/-) mice,compared with other 3 groups,IFN-γ in liver and spleen were decreased(p<0.05)and reproductive performance appeared to be impaired.Serum IFN-γ level of IL-12^(-/-)/18^(-/-) mice was significantly higher(p<0.05).It was showed that IFN-γ productions under the normal condition were independent upon IL-12 and IL-18,its expressions in various tissues were different,and optimal IFN-γ is necessary for the normal growth and development of mammals.This study is helpful for clinical cytokines therapy.Cellular & Molecular Immunology.2005;2(1):68-72.

模拟mIL-18天然生成真核表达体系的构建及生物活性初探

目的 构建模拟小鼠IL 18(mIL 18)天然生成真核表达体系 ,并探讨其与人IL 2 (hIL 2 )真核表达载体pVR10 12 hIL 2 (phIL 2 )体内外共转染对细胞免疫功能的影响。方法 分别构建小鼠IL 18前体 (mproIL 18)和小鼠IL 1β转换酶 (mICE)的真核表达载体pVR10 12 mproIL 18(pmproIL 18)和pEGFP N1 mICE(pmICE)。两者单独或共转染COS 7细胞 ,分别在mRNA和蛋白水平检测IL 18的表达 ;将pmproIL 18、pmICE和phIL 2 3种真核表达载体分别通过体内、外共转染 ,初步检测其生物学活性。结果 pmproIL 18及pmICE构建正确 ,分别转染COS 7细胞后能检测到相应mRNA表达。在pm proIL 18单独或pmproIL 18/pmICE共转染的COS 7细胞中能检测到前体和成熟 2种不同形式的mIL 18蛋白表达 ,并且mIL 18能分泌到上清 ;所分泌的mIL 18与hIL 2体外联合作用可增强小鼠脾细胞增殖能力。pmproIL 18、pmICE和phIL 2 3种真核表达载体联合肌肉注射的小鼠脾细胞体外杀伤同基因型肿瘤细胞的能力显著提高。结论 构建的模拟mIL 18天然生成的真核表达体系 (pmproIL 18/pmICE)与phIL 2共转染有可能用于肿瘤的基因治疗。

白细胞介素-18基因转染的NCI-H460肺癌细胞生物学特性研究

目的:研究IL-18基因转染的NCI-H460肺癌细胞的生物学特性。方法:设转染组(GT组)、空载体转染组(PT组)和未转染组(NT组),分别以IL-18转染的NCI-H460细胞、pcDNA3.1(+)转染的NCI-H460细胞及未转染的NCI-H460细胞为实验细胞,观察3组细胞生长情况;MTT法测定细胞增殖。Boy-den Chamber试验比较细胞侵袭能力。将3种细胞接种裸鼠,观察成瘤时间、生存时间及肿瘤大小。结果:培养第7天3组的细胞数量为GT组(5.92±0.27)×104,PT组(7.20±0.20)×104,NT组(7.09±0.12)×104,72h时A值为GT组0.97±0.08,PT组1.35±0.07,NT组1.28±0.10,3组穿透滤膜细胞数为GT组27.50±5.72,PT组38.67±6.31,NT组41.33±5.89,GT组细胞增殖及侵袭力低于PT组及NT组。3组成瘤时间为GT组(12.0±2.19)d、PT组(9.17±1.94)d、NT组(8.67±1.86)d,生存时间为GT组(51.67±7.45)d、PT组(40.17±9.83)d及NT组(37.83±10.07)d,肿瘤体积为GT组(2082.4±670.2)mm3、PT组(3893.4±316.3)mm3、NT组(3338.2±725.4)mm3,GT组细胞在裸鼠体内生长速度低于PT组及NT组。结论:IL-18基因转染的NCI-H460肺癌细胞增殖减慢,侵袭性减弱,致瘤性下降,为IL-18用于治疗恶性肿瘤奠定基础。