低分子量聚乙亚胺介导的基因转染系统及动物皮肤组织基因转染试验

将带有绿色荧光蛋白(GFP)报告基因的真核表达质粒与阳离子聚合物聚乙亚胺(PEI)结合,用肝癌细胞株CM7221实验,研究其转染效率及可能引起的细胞毒性;进一步用此PEI/DNA复合物转染小鼠皮肤组织,通过报告基因检测,研究转染基因的表达位置及持续表达时间。结果发现,低分子量PEI介导的细胞转染效率最高可达55%,转染效率与PEI结构无关,但是随着分子量的增加,转染活性略有下降。同时,随着分子量的增加,PEI对细胞的毒性也相应的加大;动物皮肤转染实验显示,转染24h后,GFP基因在皮肤组织的毛囊、汗腺、皮脂腺等处高效表达,表达可持续7天。表明低分子量PEI是低毒性、高转染效率的有用非病毒转染载体,能够在动物皮肤组织中进行基因转移,这对皮肤疾病的基因治疗具有潜在的应用价值。     

PEI在动物皮肤组织基因转化中的应用研究

用低分子量的聚乙亚胺(PEI)开发一种新的非病毒基因转染系统,为基因在皮肤组织中的有效转染提供一种可靠、廉价的方法。将带有绿色荧光蛋白报告基因(gfp)的真核表达质粒与阳离子聚合物聚乙亚胺结合,用肝癌细胞株CM7721试验,研究其转染效率及可能引起的细胞毒性;进一步转染小鼠皮肤组织,研究转染基因的表达位置及持续表达时间。结果发现,低分子量PEI介导的细胞转染效率最高可达55%,转染效率与PEI结构无关(P>0·05),但是随着PEI分子量的增加,其转染活性略有下降。同时,随着分子量的增加,PEI对细胞的毒性也相应加大;小鼠皮肤转染实验显示,转染24h后,gfp即可在皮肤组织的毛囊、汗腺、皮脂腺等处高效表达,表达可持续7~9d;进一步对皮肤用氮酮、维甲酸处理后,gfp可在皮肤组织的颗粒层细胞中高效表达。PEI是一种高效、有用的非病毒基因转染载体,能够在体外培养的动物细胞及动物皮肤组织中进行基因转移,这对皮肤疾病的基因治疗具有潜在的应用价值。     

PEI在动物皮肤组织基因转化中的应用研究

用低分子量的聚乙亚胺（PEI）开发一种新的非病毒基因转染系统,为基因在皮肤组织中的有效转染提供一种可靠、廉价的方法。将带有绿色荧光蛋白报告基因 (gfp) 的真核表达质粒与阳离子聚合物聚乙亚胺结合,用肝癌细胞株CM7721试验,研究其转染效率及可能引起的细胞毒性;进一步转染小鼠皮肤组织,研究转染基因的表达位置及持续表达时间。结果发现,低分子量PEI介导的细胞转染效率最高可达55%,转染效率与PEI结构无关（P>0.05）,但是随着PEI分子量的增加,其转染活性略有下降。同时,随着分子量的增加,PEI对细胞的毒性也相应加大;小鼠皮肤转染实验显示,转染24h后,gfp即可在皮肤组织的毛囊、汗腺、皮脂腺等处高效表达,表达可持续7～9d;进一步对皮肤用氮酮、维甲酸处理后,gfp可在皮肤组织的颗粒层细胞中高效表达。PEI是一种高效、有用的非病毒基因转染载体,能够在体外培养的动物细胞及动物皮肤组织中进行基因转移,这对皮肤疾病的基因治疗具有潜在的应用价值。     

猪瘟病毒E2基因真核表达质粒的构建及基因疫苗的研究

构建了猪瘟（ｃｌａｓｓｉｃａｌ ｓｗｉｎｅ ｆｅｖｅｒ ｖｉｒｕｓ,ＣＳＦＶ）主要保护性抗原Ｅ２基因４种不同的真核表达质粒。小鼠免疫试验表明,Ｅ２基因上不同的功能区对基因疫苗的免疫应答有很大影响,有信号肽序列的Ｅ２基因可诱导产生特异性免疫反应,且无跨膜区序列的Ｅ２基因所诱导的免疫应答反应比有跨膜区序列的强,而无信号肽序列的Ｅ２基因则不能诱导产生ＣＳＦＶ特异性的免疫反应。攻毒保护试验表明,免疫家兔最     

阳离子脂质体介导基因转染的最优化条件

阳离子脂质体介导基因转染的最优化条件王瓞林其谁（中国科学院上海生物化学研究所分子生物学国家重点实验室,上海２０００３１）关键词阳离子脂质体基因转染表达真核细胞阳离子脂质体转染的重要参数有：脂质体浓度和ＤＮＡ的浓度、细胞密度以及脂质体－ＤＮＡ复合物与细...     

含人IL—2基因的真核表达质粒的构建及其在真核细胞…

本工作用ＰＣＲ由人的外周血单个核细胞ｃＤＮＡ中获取了带有信号肽的ＩＬ－２全ｃＤＮＡ克隆,并构建了不同的表达质粒：带有ＳＶ４０启动子的以质粒为载体的ｐＳＶＫ３－ＩＬ２和以逆转录病毒为载体的ｐＬＮ－ＩＬ２系列?ｐＬＮＣＩＬ２,ｐＬＮＳＩＬ２,ｐＬＩＬ２ＳＮ,它们分别带有ＣＭＶ、ＳＶ４０和ＬＴＲ启动子。用ＤＥＡＥ－Ｄｅｘｔｒａｎ法、ＳＡ－脂质体法和电穿孔等方法分别将这些ＩＬ－２表达质粒转染入ＣＯＳ－７及     

山羊精子介导法转染外源基因影响因素及最适条件的研究

探讨山羊精子与外源DNA共孵育转染外源DNA效率的影响因素,优化精子转染程序.用DIG免疫组化方法检测和比较精子转染效率,因素为精子洗涤程度、转染缓冲液、精予活力、BSA、肝素、异种动物精浆等.离心洗涤3次以内的山羊精子DNase Ⅰ消化前、后阳性率随洗涤次数增加而显著增加(P＜0.05),而离心3次以上的转染效率略有下降;以mDM为共孵育缓冲体系可获得较高的转染效率;活力为0.55的精子转基因阳性率显著低于活力为0.9的精子(消化前、后阳性率分别为35.4±2.9%和21.8±5.3% vs 63.5±7.2%和50.3±2.8%,P＜0.os);共孵育体系中异种动物精浆可显著降低转染效率(P＜0.01),甚至与肝素可置换出已结合和内化转运到精子内的外源DNA,而共孵育体系中的BSA可抑制精子内化外源DNA.山羊共孵育法转染外源基因最适转染条件为mDM缓冲液洗涤3次后上浮收集高活力精子进行转染.     

IBDV多聚蛋白基因真核表达质粒的构建与表达

将IBDV上海超强毒株的多聚蛋白基因(vp2-4-3)克隆入真核表达载体pALTER-MAX,构建成功pALTER-MAX-VP2-4-3真核表达质粒,经纯化后,pALTER-MAX-VP2-4-3在Lipofectamie^TM2000介导下转染Vero细胞、11日龄鸡胚的绒毛尿囊膜(CAM)和肌肉注射2日龄的雏鸡,1周后,分别提取细胞或组织中的总DNA或总RNA,用DIG标记探针均可检测到阳性杂交信号;转染的Vero细胞飞片和肌肉冰冻切片,进行免疫荧光检测均呈现阳性结果;转染的鸡胚CAM匀浆上清,用兔抗IBDV超强毒的高免血清,经Dot—ELISA检测呈现阳性。表明转染后基因获得表达,表达的蛋白具有免疫反应性。     

结核分枝杆菌furA基因真核表达质粒的构建及表达

以BamH Ⅰ和Hind Ⅲ双酶切pRSET-furA,获得结核分枝杆苗铁调控基因furA,将其克隆入真核表达载体pcDNA3．1（-）,构建了重组质粒pcDNA-furA,经酶切鉴定正确后,将重组质粒以阳离子聚合物转染CHO细胞。经RT—PCR分析表明,furA可在CHO细胞中转录;用间接免疫荧光检测,表达有FurA蛋白的细胞着染。以上结果表明,通过构建结核分枝杆菌furA基因的真核表达载体pcDNA-furA,使知以基因可以在CHO细胞中表达。     

水动力转染基因在小鼠体内的长期高效表达

水动力转染技术是近年新出现的一种体内基因转染方法,可以实现目的基因在小鼠体内的高效表达,有可能作为受精卵显微注射的一种简单替代技术。但该技术的缺点是转染基因多瞬时表达,外源基因在体内高效表达的时间通常不超过1周,而且局限于肝、肾等器官,从而限制了该技术广泛应用。为了延长水动力转染基因在小鼠体内长期高效表达的时间,从而能对目的基因的体内功能进行长期研究,国外研究进行了广泛的探索,本综述了相关研究的最新进展。     

Preparation of a low molecular weight polyethylenimine for efficient cell transfection

Polyethylenimines (PEIs) of a molecular weight between 25 and about 800 kDa have successfully been used for in vitro and in vivo gene delivery approaches. Recent publications indicated that PEI molecules of lower molecular weight and a small molecular weight range are also efficient transfection reagents with a much lower cytotoxicity compared to high molecular weight PEIs. Here, we describe the application of a molecular sieve chromatography to fractionate a commercially available 25-kDa PEI. We generated three pools of PEIs with molecular weight ranges of 70-360 (I), 10-70 (II), and 0.5-10 kDa (III), respectively. We show that, in comparison with the 25-kDa PEI, pool III increased the expression of luciferase up to 100-fold and the number of transfected cells 2-3 fold. In addition, the kinetics of reporter gene expression was also much faster in pool III, compared with the 25-kDa PEI or with pools I or II. Finally, pool III showed the lowest cytotoxicity in comparison with the other PEI preparations. Thus, we provide a one-step processing of a 25-kDa PEI, resulting in a more effective and also less cytotoxic transfection reagent.     

Gene delivery with low molecular weight linear polyethylenimines

BACKGROUND: Linear polyethylenimine (LPEI) with a molecular weight (MW) of 22 kDa has been described as having a superior ability to induce gene transfer compared to its branched form. However, the transfection efficiency of the polymer cannot be enhanced beyond a certain limit due to cytotoxicity. We explored the potential of utilizing LPEIs with MWs ranging from 1.0 to 9.5 kDa to overcome this limitation. METHODS: Polyplexes of plasmid DNA encoding for the enhanced green fluorescent protein (EGFP) and various LPEIs were compared concerning their transfection efficiency and cytotoxicity in CHO-K1 and HeLa cells by flow cytometry. The involvement of endolysosomes in LPEI-mediated gene transfer was investigated by applying the proton pump inhibitor bafilomycin A1 and the lysosomotropic agent sucrose. Confocal laser scanning microscopy was applied to assess the size and shape of polyplexes under cell culture conditions, to detect their endolysosomal localization and to observe their translocation to the nucleus. RESULTS: The transfection efficiency could be altered by varying the MW and the amount of the polymer available for polyplex formation. The highest transfection efficiency (about 44%), i.e. the fraction of EGFP-positive cells, was obtained with LPEI 5.6 kDa, while the cytotoxicity remained low. The colocalization of polyplexes and endolysosomes was observed, and it appeared that the larger polyplexes escaped from the acidic organelles particularly quickly. For LPEI 5.0 and 9.0 kDa, the number of cells and nuclei that had taken up DNA after 6 hours was similar, as determined by flow cytometry. CONCLUSIONS: Our study suggests that LPEIs with low MWs are promising candidates for non-viral gene delivery, because they are more efficient and substantially less toxic than their higher MW counterparts.     

Low molecular weight polyethylenimine grafted N-maleated chitosan for gene delivery: properties and in vitro transfection studies

To develop chitosan-based efficient gene vectors, chitosans with different molecular weights were chemically modified with low molecular weight polyethylenimine. The molecular weight and composition of polyethylenimine grafted N-maleated chitosan (NMC-g-PEI) copolymers were characterized using gel permeation chromatography (GPC) and (1)H NMR, respectively. Agarose gel electrophoresis assay showed that NMC-g-PEI had good binding ability with DNA, and the particle size of the NMC-g-PEI/DNA complexes was 200-400 nm, as determined by a Zeta sizer. The nanosized complexes observed by scanning electron microscopy (SEM) exhibited a compact and spherical morphology. The NMC-g-PEI copolymers showed low cytotoxicity and good transfection activity, comparable to PEI (25 KDa) in both 293T and HeLa cell lines, except for NMC 50K-g-PEI. The results indicated that the molecular weight of NMC-g-PEI has an important effect on cytotoxicity and transfection activity, and low molecular weight NMC-g-PEI has a good potential as efficient nonviral gene vectors.     

Low molecular weight polyethylenimine for efficient transfection of human hematopoietic and umbilical cord blood-derived CD34+ cells

With the emerging role of hematopoietic stem cells as potential gene and cell therapy vehicles, there is an increasing need for safe and effective nonviral gene delivery systems. Here, we report that gene transfer and transfection efficiency in human hematopoietic and cord blood CD34+ cells can be enhanced by the use of low molecular weight polyethylenimine (PEI). PEIs of various molecular weights (800-750,000) were tested, and our results showed that the uptake of plasmid DNA by hematopoietic TF-1 cells depended on the molecular weights and the N/P ratios. Treatment with PEI 2K (m.w. 2000) at an N/P ratio of 80/1 was most effective, increasing the uptake of plasmid DNA in TF-1 cells by 23-fold relative to Lipofectamine 2000. PEI 2K-enhanced transfection was similarly observed in hematopoietic K562, murine Sca-1+, and human cord blood CD34+ cells. Notably, in human CD34+ cells, a model gene transferred with PEI 2K showed 21,043- and 513-fold higher mRNA expression levels relative to the same construct transfected without PEI or with PEI 25 K, respectively. Moreover, PEI 2K-treated TF-1 and human CD34+ cells retained good viability. Collectively, these results indicate that PEI 2K at the optimal N/P ratio might be used to safely enhance gene delivery and transfection of hematopoietic and human CD34+ stem cells.     

Inhibition of enzymatic activity of alpha-thrombin by low molecular weight synthetic inhibitor]

The effect of the organophosphoric inhibitor, SA-152, on the fibrinogen-coagulating and TAME-esterase activity of bovine alpha-thrombin was studied. The irreversible inhibition constants (k11 = 1.1 x 10(4) M-1.min-1,Ki = 0.7 x 10(-4) M, k2 = 0.8 min-1 towards the coagulating activity and kII = 0.7 x 10(4) M-1.min-1, Ki = 0.3 x 10(-4) M, k2 = 0.2 min-1 towards the esterase activity) were determined. The SA-152 inactivated alpha-thrombin was dialyzed and incubated with 0.5 M and 2.5 M NaCl and 10 mM TAME. There was no reconstitution of activity of the SA-152 modified alpha-thrombin after dialysis and treatment with high concentrations of NaCl and TAME. Heparin interactions with the anion-binding site of the high molecular weight recognition center in the alpha-thrombin molecule did not significantly influence the values of the kinetic constants for the enzyme inhibition by SA-152. This finding is consistent with the hypothesis on the irreversible binding of SA-152 in the active center of the enzyme.     

PEI-g-chitosan, a novel gene delivery system with transfection efficiency comparable to polyethylenimine in vitro and after liver administration in vivo

Polyethylenimine-graft-chitosan (PEI-g-chitosan) was synthesized by performing cationic polymerization of aziridine in the presence of water-soluble oligo-chitosan (M(n) = 3400). The absolute molecular weight and chemistry of the PEI-g-chitosan obtained were characterized using GPC, 13C and 1H NMR, respectively. The results indicated that all the amines of chitosan were grafted with oligo-PEI, and the average length of the oligo-PEI side chains was determined by the feed molar ratio of aziridne/amine in chitosan. PEI-g-chitosan of M(n) = 7400 with a polydispersity index (PDI) of 1.50, and PEI side chains of M(n) = 206 was prepared for gene delivery. Gel electrophoresis showed that DNA migration was retarded completely at a N/P ratio of 2.5/1, indicating good DNA condensation capability of PEI-g-chitosan. The sizes and the zeta-potentials of the complexes of PEI-g-chitosan/DNA were characterized. The cytotoxicity of PEI-g-chiotsan was evaluated, and the results reflected that PEI-g-chitosan had a lower cytotoxicity than PEI (25 K). Gene transfection efficiency of PEI-g-chitosan in HepG2, HeLa, and primary hepatocytes cells and after administration in the common bile duct of rat liver was determined. Remarkably, PEI-g-chitosan showed a higher transfection efficiency than that of PEI (25 K) both in vitro and in vivo. The systematic distribution and the distribution in liver of the gene expression of the complexes of PEI-chitosan/DNA were determined as well.     

The high molecular weight and the low molecular weight acid phosphatases of the frog liver and their phosphotyrosine activity

1. Two molecular weight classes of non-specific acid phosphatases (AcPases) (3.1.3.2) are present in the frog (Rana esculenta) liver: a higher molecular weight (HMW) of Mr 140,560 and a lower molecular weight (LMW) of Mr 38,180 enzyme. 2. The LMW AcPase was described earlier and the HMW AcPase of optimum pH 4.8 is shown to be a L(+)-tartrate sensitive, thermolabile, dimeric glycoenzyme slightly activated by DTT. 3. The HMW and the LMW AcPases exhibit activity for phosphotyrosine which showed similar sensitivity to various effectors as the p-nitrophenyl phosphatase activity; however, both enzymes differed substantially in this respect suggesting that they might be involved in different metabolic steps.     

Effect of the low molecular weight thymus factor on T-cells in human blood]

Lowmolecular factor of polypeptide nature (thymarin) was extracted from calf thymus. This factor differed by physical and chemical characteristics from thymosin. The percentage content of "active" T-lymphocytes increased under the effect of thymarin in the cultures of lymphoid cells obtained from healthy individuals. The total T-cell count remained unchanged. Thymarin favoured increase of the total T-lymphocyte and "active" T-lymphocyte count in the cultures of cells from patients with chronic inflammatory processes. Cellular immunity reactions were restored and the course of the main disease improved under the effect of parenteral administration of thymarin. It is supposed that T-immunity system incompetence was associated with the inadequate production of the thymus factor capable of restoring the activity of the thymus-dependent lymphocyte population.