利用烟草表达人凝血Ⅸ因子(hFIX)的研究

血友病B是凝血Ⅸ因子(hFIX)缺乏所导致的一种出血性疾病,通过输血和hFIX浓缩剂进行治疗疗效显著,但存在治疗费用高和安全隐患,因而获得安全、廉价的人凝血Ⅸ因子对血友病B治疗具有重要意义.植物系统表达外源蛋白在生产成本和安全性方面具有优势.为此,构建含人凝血Ⅸ因子基因(hFIX,2.8kb)植物双元表达载体p35s-2300∷gus∷noster,用农杆菌介导法转化烟草"百日红",通过PCR和Southern blot分析证实获得4株独立转基因植株,hFIX在转基因烟草基因组中的拷贝数为1～4个;RT-PCR和ELISA检测结果表明,hFIX在转录和翻译水平已成功表达,hFIX在转基因烟草叶片中的表达量为2.5～8.8ng/g·FW,并具有免疫活性.为利用植物系统表达hFIX的后续研究作了必要准备,也为利用植物系统表达其他药用蛋白研究提供了一些理论和实验参考.     

利用烟草表达人凝血IX因子 (hFIX)的研究

血友病B是凝血IX因子（hFIX）缺乏所导致的一种出血性疾病,通过输血和hFIX浓缩剂进行治疗疗效显著,但存在治疗费用高和安全隐患,因而获得安全、廉价的人凝血IX因子对血友病B治疗具有重要意义。植物系统表达外源蛋白在生产成本和安全性方面具有优势。为此,本研究构建含人凝血IX因子基因（hFIX,2.8kb）植物双元表达载体p35s-2300：：gus：：noster,用农杆菌介导法转化烟草 "百日红",通过PCR和Southern blot分析证实获得4株独立转基因植株, hFIX在转基因烟草基因组中的拷贝数为1-4个;RT-PCR和ELISA检测结果表明,hFIX在转录和翻译水平已成功表达,hFIX在转基因烟草叶片中的表达量为2.5~8.8ng/g·FW,并具有免疫活性。本研究为利用植物系统表达hFIX的后续研究作了必要准备,也为利用植物系统表达其他药用蛋白研究提供了一些理论和实验参考。     

利用烟草表达人凝血IX因子(hFIX)的研究

血友病B是凝血IX因子(hFIX)缺乏所导致的一种出血性疾病,通过输血和hFIX浓缩剂进行治疗疗效显著,但存在治疗费用高和安全隐患,因而获得安全、廉价的人凝血IX因子对血友病B治疗具有重要意义。植物系统表达外源蛋白在生产成本和安全性方面具有优势。为此,构建含人凝血IX因子基因(hFIX,2.8kb)植物双元表达载体p35s2300∷gus∷noster,用农杆菌介导法转化烟草“百日红”,通过PCR和Southernblot分析证实获得4株独立转基因植株,hFIX在转基因烟草基因组中的拷贝数为1～4个;RTPCR和ELISA检测结果表明,hFIX在转录和翻译水平已成功表达,hFIX在转基因烟草叶片中的表达量为2.5～8.8ng/g·FW,并具有免疫活性。为利用植物系统表达hFIX的后续研究作了必要准备,也为利用植物系统表达其他药用蛋白研究提供了一些理论和实验参考。     

人凝血IX因子基因乳腺组织特异性表达载体的构建及其在奶山羊乳腺中的分泌性表达

血友病B(Hernophilia B)是由于人凝血IX因子(hFIX)缺乏所致的一种严重出血性疾病。常规治疗方法是通过输血或输入人浓缩凝血IX园子来实现的,因此患者很容易被肝炎病毒甚至爱滋病毒感染。近年来,人们期望通过转基因动物乳腺表达并从乳汁中分离生产hFIX蛋白,以解除血友病患者的痛苦。以转基因动物的乳腺组织即乳腺生物反应器生产外源蛋白具有原核生物,酵母以及离俸真核细胞生产系统所不具备的优点：生产的外源蛋白经过体内加工和修饰,特别是真核蛋白的转译后加工(如糖基化和羧基化)．其生化特性、生物学活性与天然蛋白完全相同^[1];另外从乳汁中生产外源蛋白不需要复杂的工厂设备。因此开展人凝血IX因子乳腺生物反应器的研究具有重要的经济意义和临床应用价值。转基因动物乳腺生物反应器的关键在于外源基因乳腺组织特异性表达载体的构建。我们利用小鼠MAR元件(Matrix attachment regions)．牛的β-casein基因调控顺序,hFIX mini-gene和hFIX cDNA分别建成两种乳腺组织特异性表达载体pMCIXm和pMCIX,经SA脂质体包埋载体DNA后直接转染奶山 羊乳腺小叶,hFIX蛋白在奶山革乳汁中获得瞬间分泌性表达,最高表达量为13.7ng/ml乳汁。其中含hFIX mini-gene的表达载体在奶山羊乳汁中的表达量高于含hFIX cDNA的表达载体．表明hFIX的in-tronl能够提高该基因在活体奶山羊乳腺中的表达。A7单抗和柠檬酸钡吸附检测表明乳汁中的hFIX 蛋白羧基化和活性比率都在90％以上。以上结果肯定了载体构建的正确性．不但为研制hFIX蛋白乳腺生物反应器提供了有效的表达载体,同时也表明利用阳离子SA脂质体包埋质粒DNA直接转染活体物乳腺可以作为验证乳腺表达载体构建正确性的快速检测手段。     

人凝血因子ⅨcDNA在C2C12成肌细胞及C3H小鼠中的高效表达

以小鼠C2C12成肌细胞为对象开展血友病B基因治疗研究.除已有的XLIX,LNCIX和GlNaCIX反转录病毒载体外,又首次将微小MCK(muscle creatinekinase)增强子顺序构建到hCMV(human cytomegalovirus)启动子上游,共同控制FIXcDAN的转录.用带有上述4种载体的病毒悬液分别感染C2C12细胞后,ELISA检测结果发现,FIX蛋白离体表达水平为:G1NaMCIX>GlNaCIX>LNCIX>XLIX.其中C2C12/G1NaMCIX混合克隆高达640ng/(10~6细胞·24h).C2C12/G1NaMCIX细胞注射C3H小鼠后肢骨骼肌肉组织,人FIX蛋白持续表达35d,其中最高表达峰达206ng/mL血浆.此结果对于研究FIX cDNA在脱细胞中的表达调控以及采用成肌细胞移植途径开展血友病B基因治疗研究有重要意义.     

HGV RNA基因组感染HepG2细胞的研究*

为了观察HGV　RNA基因组在HepG2细胞中的复制和表达并建立HGV感染的细胞模型,体外转录制备HGV RNA基因组,Lipofectamin介导转染HepG2细胞。取HGV RNA阳性培养上清液传代感染HepG2细胞,采用RT-PCR、免疫组化和Western blot等技术检测HGV在HepG2细胞中的复制和表达。HepG2细胞在转染后24h便可在培养上清液中检测到HGV负链RNA,传代感染的细胞及培养上清液中可检测到HGV正、负链RNA。在90d内传代20余次,均能检测到HGV的复制。免疫组化和W     

人凝血因子IX突变型研究现状

血友病B是一种性连锁隐性遗传病,其发病机制是位于X染色体上的人凝血因子IX（hFIX）基因发生了突变,导致血浆中hFIX含量或活性大幅下降,从而使得内源性凝血途径受到阻碍,无法进行正常的凝血。本文综述了hFIX基因及其编码蛋白质的结构和功能,并分类详细论述了血友病B中发现的几种主要突变类型。其中包括奠基者效应造成的突变、调控区的突变、编码区的突变、内含子剪切位点的突变及另外两种较为特殊的突变,同时介绍了这些突变所造成的生物学效应。最后还简要介绍了一种能提高hFIX蛋白凝血活性的突变类型（第338位Arg→Ala）,并对其应用作了展望。     

人凝血因子IX突变型研究现状

血友病B是一种性连锁隐性遗传病,其发病机制是位于X染色体上的人凝血因子IX(hFIX)基因发生了突变,导致血浆中hFIX含量或活性大幅下降,从而使得内源性凝血途径受到阻碍,无法进行正常的凝血。文章综述了hFIX基因及其编码蛋白质的结构和功能,并分类详细论述了血友病B中发现的几种主要突变类型。其中包括奠基者效应造成的突变、调控区的突变、编码区的突变、内含子剪切位点的突变及另外两种较为特殊的突变,同时介绍了这些突变所造成的生物学效应。最后还简要介绍了一种能提高hFIX蛋白凝血活性的突变类型(第338位Arg→Ala),并对其应用作了展望。     

阳离子脂质体介导hFL真核表达载体在骨髓基质细胞系中的表达

目的阳离子脂质体介导hFL真核表达载体pIRESlneo/hFL转染人骨髓基质细胞系HFCL细胞,观察hFL在HFCL细胞中的表达.方法以阳离子脂质体介导法将重组真核表达载体pIRESlneo/hFL导入人骨髓基质细胞系HFCL细胞,G418筛选获得的阳性细胞以Southemblot和Northernblot分别检测其基因组DNA整合和mRNA转录,Westernblot检测其蛋白表达,ELISA及人脐血CD34+细胞增殖实验检测其蛋白表达量和活性.结果hFL基因己整合到靶细胞HFCL基因组DNA中,在mRNA和蛋白质水平上均可检测到其表达,ELISA法测得hFL的表达量为(60.3±0.3)ng.106Cell-1@d-1,分泌量在细胞传代30次后仍保持稳定,并且表达的hFL具有良好的生物学活性.结论阳离子脂质体介导的hFL真核表达载体在人骨髓基质细胞系HFCL中获得持续稳定表达,并具有良好的生物学活性.为转基因骨髓基质细胞移植促进造血重建的体内动物实验研究奠定了基础.     

人凝血因子Ⅸ突变型研究现状

血友病B是一种性连锁隐性遗传病,其发病机制是位于X染色体上的人凝血因子Ⅸ(hFIX)基因发生了突变,导致血浆中hFIX含量或活性大幅下降,从而使得内源性凝血途径受到阻碍,无法进行正常的凝血.文章综述了hFIX基因及其编码蛋白质的结构和功能,并分类详细论述了血友病B中发现的几种主要突变类型.其中包括奠基者效应造成的突变、调控区的突变、编码区的突变、内含子剪切位点的突变及另外两种较为特殊的突变,同时介绍了这些突变所造成的生物学效应.最后还简要介绍了一种能提高hFIX蛋白凝血活性的突变类型(第338位Arg→Ala),并对其应用作了展望.     

Transgenic Mice Can Express Mutant Human Coagulation Factor IX with Higher Level of Clotting Activity

To improve the available values of transgenic animals, we produced a mutant human coagulation factor IX minigene (including cDNA and intron I) with arginine at 338 changed to alanine (R338A-hFIX) by using a direct mutation technique. The R338A-hFIX minigene was then cloned into a plasmid carrying the goat β-casein promoter to get a mammary gland-specific expression vector. The clotting activity in the supernatant of the transfected HC-11 cells increased to approximately three times more than that of wild-type hFIX. Nine transgenic mice (three females and six males) were produced, and the copy number of the foreign gene was very different, ranging from 1 to 43 in different lines. ELISA, Western blot, and clotting assay experiments showed that the transgenic mice could express R338A-hFIX, showing higher average levels of clotting activity than wild-type hFIX in the milk (103.76% vs. 49.95%). The highest concentration and clotting activity of hFIX reached 26 μg/mL and 1287% in one founder (F₀-7), which was over 10 times higher than that in human plasma. Furthermore, RT-PCR, APTT assay, and histological analysis indicated that hFIX was expressed specifically in the mammary gland without affecting the intrinsic coagulation pathway and physiologic performance of the local tissue.     

Expression and regulation of hFIX minigene and cDNA driven by β-casein gene in mouse mammary gland

Mammary gland specific expression vectors for human clotting factor IX (hFIX) and LacZ reporter gene driven by bovine β-casein gene were constructed. Vectors were packaged by stearylamine (SA) liposome and were transferred to lactating mice via tail vein. Both hFIX and Lac2 gene could be expressed in the mammary gland of the treated mice. The highest production of hFIX protein was 80.28 ng per mL milk, and more than 85% of hFIX protein appeared to be γ-carboxylation and biologically active. The results suggested that the 2.0 kb sequence of β-casein gene including promoter, exon 1 was effective to drive hFIX gene expression in mammary gland and intron 1 of β-casein gene had an effect on the tissue specific expression. The expression level in mouse milk injected with hFIX minigene vector containing hFIX endogenous intron 1 was increased by above 3 times of that injected with hFIX cDNA vector. Project supported by the State High Technology Development Program and Shanghai Science and Technology Commission.     

Differentiation in human amniotic fluid cell cultures: Chorionic gonadotropin production

Summary Two of the distinguishable cell classes subcultured from human amniotic fluid were examined for their capability to produce human chorionic gonadotropin (hCG) as determined by radioimmunoassay. The class that predominates in most cultures used for prenatal genetic diagnosis, previously termed AF (for amniotic fluid), secretes hCG into the culture medium. Dermal fibroblasts do not, nor does another type of cultured cell from amniotic fluid, previously termed F because of a resemblance to fibroblasts. Primary AF cultures produce more hCG than do subcultures. Evidence that this hormone is intact hCG is provided by its immunoreactivity with antisera raised against the β-subunit and against the intact molecule of hCG. Furthermore, a dose-response curve for hormone in culture medium is parallel to that of highly purified intact hCG. It is postulated that AF cultures are derived from fetal membranes and retain properties of trophoblast. Research supported by Grand HD 11379 from the National Institutes of Health.     

Citrullinemia: prenatal diagnosis of an affected fetus.

We monitored a pregnancy in a family at risk for citrullinemia due to argininosuccinic acid (ASA) synthetase deficiency. ASA synthetase activity in cultured epithelioid amniotic fluid cells from the fetus at risk was less than 2% of control epithelioid amniotic fluid cell activity. An increased concentration of citrulline was found in the at-risk amniotic fluid (0.14 mumol/ml) as compared with fluid from six controls and one at-risk but unaffected pregnancy (trace). The pregnancy was terminated, and the in utero diagnosis was confirmed by assay of ASA synthetase activity in cultured fetal skin fibroblasts (4.4% of control activity). In addition, all five fetal tissues studied had significant accumulation of citrulline, whereas control fetal tissues had none. These data provide evidence that, if precise control is maintained over tissue culture variables, citrullinemia can be diagnosed successfully in utero by microassay of ASA synthetase activity in cultured amniotic fluid cells. They also suggest that amniotic fluid citrulline concentrations provide strong adjunctive evidence for this prenatal diagnosis.     

High expression of human clotting factor IX cDNA in myoblasts C2C12 cells and C3H mice

Mouse myoblast C2C12 cell was used as target cell for gene transfer study of human clotting factor IX (hFIX) cDNA. In addition to the previously constructed retroviral vectors XLIX, LNCIX and GINaCIX, GlNaMCIX with hFIX driven by muscle creatine kinase (MCK) enhancer and human cytomegalovirus (CMV) was constructed, based on the retroviral vector GINa. These four retroviral vectors were used to transduce mouse my-oblasts C2C12. With ELISA assays, it has been found that the expression levels of human clotting factor IX detected in those transduced C2C12 cells are GlNaMCIX>GlNaCIX> LNCIX>XLIX. Mixed colonal cells transduced with GlNaMCIX expressed hFIX protein at the level of 640 ng/106 cell every 24 h. The modified C2C12 cells transduced with GlNaMCIX were implanted into skeletal muscle of the hindlegs of C3H mice; a stable expression of hFIX was detected and lasted for 35 d, with a maximum level of 206 ng/mL plasma. The regulation of hFIX cDNA expression in myoblasts was discussed and it was strongly sug     

Increment of hFIX expression with endogenous intron 1 in Vitro

This paper probes into the feasibility of increasing expression level of hFIX gene with endogenous intron 1 sequence.hFIX minigene was obtained with middle sequence truncated intron 1 inserted into the relative site of hFIX cDNA,and plasmid vector pKG5i‘IX,retroviral vector G1NaCi‘IX were constructed.These vectors were transduced into target cells of PA317,C2C12,primary rabbit skin fibroblasts (RSF) and primary human skin fibroblasts (HSF).The expression level of mixed colonies are PA317/pKG5i‘IX,151 ng/10^6 cells/24h;PA317/G1NaCi‘IX,308 ng/10^6 cells/24 h;C2C12/G1NaCi‘IX,186 ng/10^6 cells/24 h;RSF/G1NaCi‘IX,1929 ng/10^6 cells/24 h;HSF/G1NaCi‘IX,1646 ng/10^6 cells/24 h.These results indicated that hFIX minigene with intron l is able to increase the expression level to about 3 times of that of hFIX cDNA.Meanwhile,in order to study the application of hFIX minigene in the retroviral-mediated gene transfer system and refrain from intron splicing during viral production,a retroviral vector G1NaCi‘IXR with reversely inserted hFIX minigene expression cassette was constructed.The expression level of reverse constructor in PA317 cells was 390 ng/10^6 cells/24 h with 79% of bioactivity.PCR detection of HT/G1NaCi‘IXR cells infected with PA317/G1NaCi‘IXR supernatant confirmed the existence of intron 1 sequence.These results suggested that expression vector with forward-inserted intronl-carrying hFIX expression cassette can be used in directed gene transfer,but when using the retroviral-mediated gene transfer system,reversely-inserted intronl-carrying hFIX expression cassette should be considered.     

Clonal amniotic fluid-derived stem cells express characteristics of both mesenchymal and neural stem cells

Recent evidence has shown that amniotic fluid may be a novel source of fetal stem cells for therapeutic transplantation. We previously developed a two-stage culture protocol to isolate a population of amniotic fluid-derived mesenchymal stem cells (AFMSCs) from second-trimester amniocentesis. AFMSCs maintain the capacity to differentiate into multiple mesenchymal lineages and neuron-like cells. It is unclear whether amniotic fluid contains heterogeneous populations of stem cells or a subpopulation of primitive stem cells that are similar to marrow stromal cells showing the behavior of neural progenitors. In this study, we showed a subpopulation of amniotic fluid-derived stem cells (AF-SCs) at the single-cell level by limiting dilution. We found that NANOG- and POU5F1 (also known as OCT4)-expressing cells still existed in the expanded single cell-derived AF-SCs. Aside from the common mesenchymal characteristics, these clonal AF-SCs also exhibit multiple phenotypes of neural-derived cells such as NES, TUBB3, NEFH, NEUNA60, GALC, and GFAP expressions both before and after neural induction. Most importantly, HPLC analysis showed the evidence of dopamine release in the extract of dopaminergic-induced clonal AF-SCs. The results of this study suggest that besides being an easily accessible and expandable source of fetal stem cells, amniotic fluid will provide a promising source of neural progenitor cells that may be used in future cellular therapies for neurodegenerative diseases and nervous system injuries.     

一种新型生物反应器在造血干/祖细胞体外扩增中的应用

针对造血干/祖细胞体外扩增对培养环境的需求, 结合静/动态培养的特点, 开发了一种新型的生物反应器用于造血干/祖细胞的体外扩增。在该生物反应器内, 采用SCF+TPO+Flt-3细胞因子组合, 比较了静态和循环培养两种方式体外扩增脐血CD34+细胞的效果。培养7 d后, 总细胞分别扩增了(13.86 ± 4.26)和(7.23 ± 2.67)倍, 显示静态培养有利于总细胞的扩增; CD34+细胞扩增倍数、培养物中CD34+细胞含量均相近, 无显著性差异; 而CD34+CD38-细胞扩增倍数以及培养物中CD34+CD38?细胞的百分含量分别为(1.82 ± 0.58)和(3.90 ± 0.85)倍以及(9.45 ± 4.85)和(37.47 ± 14.06)%, 循环培养明显高于静态培养。可见, 在该生物反应器内, 采用静态和循环两种培养方式, 均能实现造血干/祖细胞的体外扩增, 但静态培养促使造血干细胞向定向祖细胞分化, 而循环培养则更有利于早期造血干细胞的扩增。     

一种新型生物反应器在造血干/祖细胞体外扩增中的应用

针对造血干/祖细胞体外扩增对培养环境的需求, 结合静/动态培养的特点, 开发了一种新型的生物反应器用于造血干/祖细胞的体外扩增.在该生物反应器内, 采用SCF TPO Flt-3细胞因子组合, 比较了静态和循环培养两种方式体外扩增脐血CD34 细胞的效果.培养7 d后, 总细胞分别扩增了(13.86 ± 4.26)和(7.23 ± 2.67)倍, 显示静态培养有利于总细胞的扩增; CD34 细胞扩增倍数、培养物中CD34 细胞含量均相近, 无显著性差异; 而CD34 CD38-细胞扩增倍数以及培养物中CD34 CD38-细胞的百分含量分别为(1.82 ± 0.58)和(3.90 ± 0.85)倍以及(9.45 ± 4.85)和(37.47 ± 14.06)%, 循环培养明显高于静态培养.可见, 在该生物反应器内, 采用静态和循环两种培养方式, 均能实现造血干/祖细胞的体外扩增, 但静态培养促使造血干细胞向定向祖细胞分化, 而循环培养则更有利于早期造血干细胞的扩增.