Egr-1基因调控序列连接OSM cDNA表达质粒的构建及其在黑色素瘤细胞中的表达

ＯＳＭ是一种对黑色素瘤细胞显示抑制作用的细胞因子．为进行ＯＳＭ针对黑色素瘤的基因－放射治疗研究,构建了小鼠Ｅｇｒ－１基因调控序列引导入ＯＳＭｃＤＮＡ真核表达质粒（ｐＥＯ）,ｐＥＯ质粒转染小鼠Ｂ－１６黑色素瘤细胞,经Ｇ４１８和抗人ＯＳＭ抗体的筛选,获得了稳定表达ＯＳＭ的克隆细胞（ｐＥＯ－１细胞）,ＯＳＭ表达量可达５．９７ｎｇ每１０５细胞天,分子量为３２ｋＤ．ｐＥＯ－１细胞用一定浓度Ｈ２Ｏ２处理后ＯＳＭ表达量可提高６２％,表明ｐＥＯ重组质粒可在氧自由基的刺激作用下增强ＯＳＭ表达     

人白细胞介素—2基因在人骨肉瘤细胞系内表达

从ｐＨＩＧ５３质粒内切下人白细胞介素－２ｃＤＮＡ基因,并经中间一ｐＳＰ７２转换成与ｐＤＯＲ－ｎｅｏ载体相区域的酶切位点,然后将ＩＬ－２ｃＤＮＡ定向连接入ｐＤＯＲ－ｎｅｏ载体,构建成功人ＩＬ－２逆转录病毒载体,经脂质体民入人骨肉瘤细胞系Ｍａ中,经Ｇ４１８筛选后测转基因肿瘤细胞培养上清中ＩＬ－２表达量,每１×１０＾５细胞２４ｈＩＬ－２表达量为５０－８００Ｕ,为骨肉瘤的基因治疗创造条件。     

小鼠4.5S RNA逆转座子对Luc基因表达的影响

利用ＲＴ－ＰＣＲ方法,从小鼠肝脏组织总ＲＮＡ中扩增出４．５ＳＲＮＡ的ｃＤＮＡ。该ｃＤＮＡ被克隆到ｐＧＥＭ３Ｚｆ（＋）质粒上,酶切鉴定并测序。然后将该序列插入以Ｌｕｃ基因作为报道基因的表达载体ｐＳＶｌｕｃ２０的ＰｖｕⅡ位点,构建了含４．２ＳＲＮＡ逆转座子的表达载体ｐＳＶｌｕｃ２０－４．５Ｓ。脂质转染法将表达载体导入小鼠骨髓瘤细胞ＮＳ－１、ＳＰ２／０和人乳腺癌细胞Ｂｃａ６１。结果表明,小鼠４．５ＳＲＮ     

c－mpl原癌基因编码促血小板生成素受体

ｃ－ｍｐｌ原癌基因编码促血小板生成素受体郭树华,贺福初,吴祖泽（北京放射医学研究所,北京１００８５０）ｃ－ｍｐｌ原癌基因是ｖ－ｍｐｌ（ｍｙｅｌｏＰｒｏｌｉｆｅｒａｔｉｖｅｌｅｕｋｅｍｉａｖｉｒｕｓ,ＭＰＬＶ）的正常细胞的对应物．人的全长ｃ－ｍｐｌｃＤ...     

hBMP—2cDNA在COS细胞和小鼠肌肉中的表达

研究了骨形态发生蛋白ＢＭＰ－２ｃＤＮＡ在ＣＯＳ细胞和小鼠肌肉中的表达的情况,从ｐＳＰＳ６５ＢＭＰ－２质粒中回收ＢＭＰ－２ｃＤＮＡ,删除５端的非翻译序列,插入ｐＳＶＬ载体中,构建了含有ＢＭＰ－２全长编码序列的重组表达质粒ｐＳＶＬＢＭＰ－２将表达质粒导入ＣＯＳ－７细胞中,细胞ＲＮＡ点杂交结果表明,转染ＢＭＰ－２基因的细胞内ＢＭＰ－２的ｍＲＮＡ水平明显升高,细胞培养上清的ＥＬＩＳＡ显示,转染ＢＭＰ－２ｃ     

Epstein-Barr病毒膜抗原基因免疫的研究

将Ｅｐｓｔｅｉｎ－Ｂａｒ病毒（ＥＢＶ）膜抗原（ＭＡ）ＢＬＬＦ１基因,插入含有ＣＭＶ启动子的真核表达载体ｐｃＤＮＡ３下游ＢａｍＨＩ位点,构建成真核表达质粒ｐｃＤＮＡ３－ＭＡ。将纯化的ＤＮＡ注射Ｂａｌｂ／ｃ小鼠股四头肌。经免疫的动物产生抗ＥＢ病毒ＭＡ特异性的抗体和中和抗体,依赖抗体细胞介导的细胞毒作用（ＡＤＣＣ）,特异性Ｔ淋巴细胞增生性反应及细胞毒性Ｔ淋巴细胞（ＣＴＬ）杀伤作用。基因免疫与基因－蛋白联合免疫效果相似。不同启动子控制下的ＭＡ基因,诱发小鼠免疫应答无明显差异。     

小鼠金属硫蛋白 Ⅰ cDNA编码序列的克隆及其在昆虫细胞中的表达

将质粒ｐＢＸ－ＭＴ上的小鼠ＭＴ－ⅠｃＤＮＡ片段切下作为模板,通过ＰＣＲ方法删除该片段的非编码序列,将编码序列克隆到质粒ｐＢＳ－ＳＫ中,经ＤＮＡ序列测定后证明其克隆序列正确．再将ＭＴ－ⅠｃＤＮＡ编码序列插入到转移载体ｐＢａｃＰＡＫ８的ＢａｍＨⅠ和ＥｃｏＲⅠ位点之间,通过磷酸钙／ＤＮＡ共转染方法将其导入昆虫细胞Ｓｆ９中,以Ｗｅｓｔｅｒｎｂｌｏｔ和ＤｏｔＥＩＡ方法对表达产物进行了检测,表达量为１ｍｇ／Ｌ     

用5-Fu治疗MT/p210bcr-abl转基因小鼠的研究

以５－氟脲嘧啶（５－ｆｌｕｏｒｏｕｒａｃｉｌ,５－Ｆｕ）腹腔注射治疗了１２只携有金属硫蛋白（Ｍｅｔａｌｏｔｈｉｏｎｅｉｎ,ＭＴ）启动子和增强子序列、ｂｃｒ－ａｂｌｃＤＮＡ（ｐ２１０）序列及ＳＶ４０剪切和Ｐｏｌｙ（Ａ）信号序列的转基因慢粒白血病（ｃｈｒｏｎｉｃｍｙｅｌｏｉｄｌｅｕｋｅｍｉ－ａ,ＣＭＬ）ＭＴ／ｐ２１０ｂｃｒ－ａｂｌ小鼠,于治疗的第５ｄ及第１０ｄ从不同脏器提取总ＲＮＡ、ＤＮＡ及蛋白质,分别进行ＰＣＲ分析、ＲＴ－ＰＣＲ检测被转移基因的表达水平及免疫沉淀法分析ｐ２１０ｂｃｒ－ａｂｌ转基因产物的激酶活性．结果表明,被转移基因在脾脏和骨髓中表达水平较高,胸腺和肾脏中呈低水平表达．５－Ｆｕ活体治疗１０ｄ后,被转移基因的表达水平及其表达产物的激酶活性均被明显抑制     

hBMP－2cDNA在COS细胞和小鼠肌肉中的表达

研究了骨形态发生蛋白ＢＭＰ－２ｃＤＮＡ在ＣＯＳ细胞和小鼠肌肉中的表达的情况,从ｐＳＰＳ６５ＢＭＰ－２质粒中回收ＢＭＰ－２ｃＤＮＡ,删除５＇端的非翻译序列,插入ｐＳＶＬ载体中,构建了含有ＢＭＰ－２全长编码序列的重组表达质粒ｐＳＶＬＢＭＰ－２。将表达质粒导入ＣＯＳ－７细胞中,细胞ＲＮＡ点杂交结果表明,转染ＢＭＰ－２基因的细胞内ＢＭＰ－２的ｍＲＮＡ水平明显升高;细胞培养上清的ＥＬＩＳＡ显示,转染ＢＭＰ－２ｃＤＮＡ后,细胞分泌产生的ＢＭＰ－２显著增加。小鼠实验发现,在肌肉内用注射法导入ＢＭＰ－２重组质粒后,局部组织内ＢＭＰ－２的ｍＲＮＡ转录水平也明显提高。     

小鼠白细胞介素12双顺反子真核表达载体的构建及其在COS-7细胞中的表达

克隆小鼠白细胞介素１２（ＩＬ－１２）ｐ４０及ｐ３５ｃＤＮＡ,并构建同时含ｍＩＬ－１２ｐ４０和ｐ３５ｃＤＮＡ的双顺反子真核表达载体及其在哺乳动物细胞中的表达．白细胞介素１２是由巨噬细胞,树突状细胞等抗原提呈细胞产生的一种异二聚体细胞因子,对机体的细胞免疫功能起着重要的调节作用．利用脂多糖（１００ｐｇ／ｍｌ）和小鼠重组干扰素（ＩＦＮ－γ５００Ｕ／ｍｌ）体外联合刺激小鼠腹腔巨噬细胞,从中提取总ＲＮＡ,经ＲＴ－ＰＣＲ扩增出含信号肽的小鼠白细胞介素１２（ｍＩＬ－１２）ｐ４０及ｐ３５全长ｃＤ－ＮＡ．ＰＣＲ产物经酶切后,分别克隆至ｐＢｌｕｅｓｃｒｉｐｔⅡＳＫ载体中,序列测定结果与文献报道序列一致．然后利用脊髓灰质炎（Ｐｏｌｉｏ）病毒内核糖体进入位点（ＩＲＥＳ）连接ｍＩＬ－１２ｐ４０及ｐ３５ｃＤＮＡ,亚克隆至ｐｃＤＮＡ３载体中,构建成含ｍＩＬ－１２ｐ４０及ｐ３５ｃＤＮＡ双顺反子真核表达载体,即ｐｃＤＮＡ３／ｍＩＬ－１２,ｐ４０及ｐ３５ｃＤＮＡ同时受ｐｃＤＮＡ３中ｈＣＭＶ启动子驱动,将ｐ４０及ｐ３５转录至同一ｍＲ－ＮＡ上．通过ＬｉｐｏｆｅｃｔＡＭＩＮＥ将ｐｃＤＮＡ３／ｍＩＬ－１２转染ＣＯＳ－７细胞,７２ｈ收集培养上清,测定ｍ     

人促血小板生成素受体c-Mpl编码区全长cDNA的克隆及其稳定表达的细胞株的构建

以人HEL细胞总RNA为模板,采用RT-PCR方法扩增了人促血小板生成素受体c-Mpl编码区全长1.9kb cDNA,测序结果表明与已报道的序列一致。然后构建了c-mpl的pcDNA3表达载体pcMPL,转染不表达cmpl的K562细胞后,经G418抗性筛选,Northern blot和Southern blot检测证实获得稳定表达cmpl的细胞株。为进一步研究cMpl的生物学功能提供有用的实验材料。     

Control of thrombopoietin-induced megakaryocytic differentiation by the mitogen-activated protein kinase pathway.

Thrombopoietin (TPO) is the major regulator of both growth and differentiation of megakaryocytes. We previously showed that both functions can be generated by TPO in the megakaryoblastic cell line UT7, in which murine Mpl was introduced, and are independently controlled by distinct regions of the cytoplasmic domain of Mpl. Particularly, residues 71 to 94 of this domain (deleted in the mutant mpl delta3) were found to be required for megakaryocytic maturation but dispensable for proliferation. We show here that TPO-induced differentiation in UT7 cells is tightly dependent on a strong, long-lasting activation of the mitogen-activated protein kinase (MAPK) pathway. Indeed, (i) in UT7-mpl cells, TPO induced a strong activation of extracellular signal-regulated kinases (ERK) which was persistent until at least 4 days in TPO-containing medium; (ii) a specific MAPK kinase (MEK) inhibitor inhibited TPO-induced megakaryocytic gene expression; (iii) the Mpl mutant mpl delta3, which displayed no maturation activity, transduced only a weak and transient ERK activation in UT7 cells; and (iv) TPO-induced megakaryocytic differentiation in UT7-mpl delta3 cells was partially restored by expression of a constitutively activated mutant of MEK. The capacity of TPO to trigger a strong and prolonged MAPK signal depended on the cell in which Mpl was introduced. In BAF3-mpl cells, TPO triggered a weak and transient ERK activation, similar to that induced in UT7-mpl delta3 cells. In these cells, no difference in MAPK activation was found between normal Mpl and mpl delta3. Thus, depending on the cellular context, several distinct regions of the cytoplasmic domain of Mpl and signaling pathways may contribute to generate quantitative variations in MAPK activation.     

大鼠催乳素基因真核细胞可表达性质粒的构建及应用研究

７３５ｂｐ的ＰＲＬｃＤＮＡ片段从质粒ＰＲＬ－ＳＰ６５＃１中回收后,用粘性末端连接法将其重组到真核表达载体ｐｃＤＮＡ３上,筛选出正向连接重组体ｐｃＤＮＡ３－ＰＲＬＳ和反向连接重组体ｐｃＤＮＡ３－ＰＲＬＡＳ。将重组体ｐｃＤＮＡ３－ＰＲＬｓ和空载体ｐｃＤＮＡ３分别转入ＮＩＨ３Ｔ３细胞系,用Ｇ４１８筛选出阳性细胞后与未转染的ＮＩＨ３Ｔ３细胞在加Ｅ２和不加Ｅ２的情况下,用原位杂交的方法,分别用ＰＲＬｃＤＮＡ探针和原癌基因ｃ－Ｈ－ｒａｓｃＤＮＡ探针进行检测,未转染的ＮＩＨ３Ｔ３细胞在加Ｅ２和不加Ｅ２时都几乎无催乳素基因的表达,同样,转入空载体的ＮＩＨ３Ｔ３细胞也无ＰＲＬ的表达,而转入重组体ｐｃＤＮＡ３－ＰＲＬＳ的ＮＩＨ３Ｔ３细胞则有大量的ＰＲＬ基因的表达,与对照组相比有显著差异（Ｐ＜０．０１）。正常和转入空载体的ＮＩＨ３Ｔ３细胞有一定程度的原癌基因ｃ－Ｈ－ｒａｓ的表达,当分别加入Ｅ２和转入重组体ｐｃＤＮＡ３－ＰＲＬＳ后,ＮＩＨ３Ｔ３细胞中的ｃ－Ｈ－ｒａｓ基因表达水平都显著升高（Ｐ＜０．０５）。     

Murine c-mpl: a member of the hematopoietic growth factor receptor superfamily that transduces a proliferative signal.

The murine myeloproliferative leukemia virus has previously been shown to contain a fragment of the coding region of the c-mpl gene, a member of the cytokine receptor superfamily. We have isolated cDNA and genomic clones encoding murine c-mpl and localized the c-mpl gene to mouse chromosome 4. Since some members of this superfamily function by transducing a proliferative signal and since the putative ligand of mpl is unknown, we have generated a chimeric receptor to test the functional potential of mpl. The chimera consists of the extracellular domain of the human interleukin-4 receptor and the cytoplasmic domain of mpl. A mouse hematopoietic cell line transfected with this construct proliferates in response to human interleukin-4, thereby demonstrating that the cytoplasmic domain of mpl contains all elements necessary to transmit a growth stimulatory signal. In addition, we show that 25-40% of mpl mRNA found in the spleen corresponds to a novel truncated and potentially soluble isoform of mpl and that both full-length and truncated forms of mpl protein can be immunoprecipitated from lysates of transfected COS cells. Interestingly, however, although the truncated form of the receptor possesses a functional signal sequence and lacks a transmembrane domain, it is not detected in the culture media of transfected cells.     

P48L和D74N突变对p16基因功能的影响

应用DNA聚合酶链式反应(PCR)技术,对p16抑癌基因(CDKN2)进行体外定点突变,在p16cDNA中引入第48位密码子CCG(Pro)→CTG(Leu)和第74位密码子GAC(Asp)→AAC(Asn)突变,构建了p16-P48L和p16-D74N突变体。野生型和突变型p16 cDNA克隆于pcDNA3构建pCMV-p16、pCMV-p16P48L和pCMV-p16D74N真核表达载体,导入纯合缺失p16基因的人肺癌细胞株H460,经RNA点杂交、RNA印迹和细胞免疫化学染色,检测到P16表达。通过比较表达野生型和突变型P16的H460细胞在~3H-TdR掺入及细胞所在周期的差异,证实P16表达抑制细胞进入S期,而P48L和D74N突变体对细胞进入S期没有什么影响,提示P48L和D74N突变导致P16蛋白功能丧失。     

异种器官移植用血管内皮细胞特异表达人CD59重组基因的构建

PCR插入法将人细胞间粘附分子（ICAM－2）启动子、人CD59－enhancer克隆到human CD59cDNA-pcDNA3表达质粒中,进行序列测定及分析。成功地构建了异种器官移植用血管内皮细胞特异表达人CD59重组基因,提供了CD59重组基因用于转基因动物的研究。     

人sTNFR1基因的克隆以及在NIH3T3细胞中的稳定表达

以He1a细胞的总RNA为模板,用RT—PCR方法扩增sTNFR1全编码区基因片段,构建含有目的片段的T载体克隆及真核表达载体pcDNA3．1（-）重组质粒亚克隆,将重组质粒和脂质体共同转染NIH3T3细胞系,G418筛选稳定转染细胞株．经核苷酸序列测序和酶切鉴定,成功构建了pcDNA3．1（-）-sTNFR1真核表达质粒,脂质体法建立了高效表达sTNFRI的稳定转染细胞系,并经RT—PCR和Western Blotting鉴定．人sTNFR1基因能在NIH3T3细胞系中稳定表达,为今后的研究打下了基础．     

H1亚型猪流感病毒血凝素基因在昆虫细胞中的表达及其间接

根据GenBank发表的H1亚型猪流感HA基因序列设计引物,扩增出HA基因片段.将其克隆到pFastBacGP67B杆状病毒载体上,筛选阳性重组转座载体pFastBacGP67B-H1,转化含有杆状病毒穿梭载体(bacmid)的DH10Bac感受态细胞,构建杆状病毒表达载体获得重组转座子(rBacmid-H1),在脂质体介导下转染sf9昆虫细胞,获得重组杆状病毒(rBV-H1),再感染细胞,收获目的蛋白.通过血凝试验、免疫印迹法、免疫组化分析表明该蛋白得到表达,且具有良好的生物学活性.利用表达的蛋白作为猪流感间接ELISA的抗原,初步建立H1亚型猪流感的间接ELISA检测方法,并对内蒙古、辽宁和黑龙江等地送检的93份猪血清进行了检测,阳性率为31.18%,为研制开发快速、准确、简便的H1亚型猪流感鉴别诊断试剂盒奠定基础.     

人补体调节蛋白DAF、MCP在哺乳动物细胞中的共表达及协同作用研究

利用双启动子构建含人补体调节蛋白DAF和MCP cDNA的双顺反子重组表达载体pcDNA3-DAFMCP-DP, 以磷酸钙沉淀法转染NIH3T3细胞, 用G418筛选获得NIH3T3 pcDNA3-DAFMCP-DP转化细胞。PCR实验结果显示人补体调节蛋白基因DAF和MCP整合在转化的异源细胞的染色体上。RT-PCR和Western blot印迹实验分别从RNA水平和蛋白质水平证实了人补体调节蛋白分子DAF和MCP在细胞系中皆获得同步表达。检测连续传代30次的NIH3T3 pcDNA3-DAFMCP-DP结果表明人DAF和MCP基因仍稳定整合在细胞基因组中, 并未随着传代而丢失, 为稳定的转双基因细胞系。补体依赖的细胞毒反应表明, pcDNA3-DAFMCP-DP转染细胞系由于DAF和MCP的共表达获得较DAF或MCP单一表达时更强的保护能力, 能更好地抑制人补体依赖的细胞毒作用的发生, 保护宿主细胞免受人补体的攻击。以上结果表明, DAF和MCP双基因重组表达载体实现了人补体调节蛋白基因高效转移和高水平共表达, 为获得表达多种人补体调节蛋白的理想供体提供了有效策略。而且共表达的DAF和MCP具有协同效应, 能更有效地阻止补体激活造成的细胞损伤, 在克服超急性排斥反应的基因治疗中具有潜在的临床应用价值。     

In vitro and in vivo transfection and expression of plasmid-based non-viral vector for erythropoietin gene therapy

A non-viral gene therapy vector, pcDNA3-EPO, was constructed by subcloning erythropoietin (EPO) cDNA into plasmid pcDNA3. After liposome-mediated transfection of the NIH 3T3 cells in vitro, EPO expression in the culture medium was detected by ELISA and amounted to 1.25 ± 0.3 IU ml^–1. The biological activity of this EPO in the medium was detected after intramuscular injection of BALB/c mice. PCR of genomic DNA and RT-PCR of total RNA also confirmed that the plasmid pcDNA3-EPO had been transfected into the cells. A pool of pcDNA3-EPO transfectants, which stably expressed EPO, was obtained by G418 selection. When pcDNA3-EPO was combined into liposomes and intramuscularly injected into BALB/c mice, the reticulocyte ratio in the positive mice was three times higher than that in the control mice. In vivo expression was maintained in mice for at least one month.