基因枪在大鼠闭塞性血管病基因治疗中的应用

探讨利用基因枪技术转移肝细胞生长因子基因治疗大鼠肢体闭塞性血管病的可行性,构建了携带人肝细胞生长因子（HGF）基因的重组真核表达载体（pUDKH),在制备好大鼠下肢闭塞性血管病模型后,通过基因枪或肌肉直接注射法,向局部缺血部位肌肉中转移pUDKH,每只5ug(基因枪）和12ug(肌肉注射）,应用常规组织病理切片（H．E．染色）及免疫组织化学方法观察血管形成及基因表达,转移pUDKH后第10天,用基因枪和直接注射法转移的局部肌肉组织的HGF的表达明显高于转移空白质粒（pUDK)的对照组,pUDKH组可见明显的小血管新生,而pUKD组至20天时仍未观察到或仅见到极少量的新生血管,基因枪与肌肉注射两组相比血管密度无明显差异,采用基因枪直接转移pUDKH裸露质粒子肢体缺血局部的方法是可行的,转移的基因可在局部有效表达,达到促进血管形成的预期目的。     

血管内皮细胞生长因子研究进展

从不同侧面阐述了血管内皮细胞生长因子（VEGF）在新生血管形成中的作用.VEGF诱导新生血管形成,具有血管渗透性,是新生血管形成的主要调控者之一.VEGF mRNA不同剪接,形成5种VEGF变异体(isoform)即VEGF121-206.VEGF诱导新生血管的调控过程、拮抗VEGF成为大家竞相研究的领域.     

血管内皮细胞生长因子促进成骨作用的研究进展

骨组织的生长和血供密切相关 ,血管内皮细胞生长因子 (VEGF)被公认为是诱导血管生成作用最强的一种细胞因子 ,其自身也和骨形成有着直接的关系。通过对VEGF及其受体分子结构、其在骨发育和骨损伤修复中所起作用、以及目前常见应用方式的相关研究作一系统性回顾 ;阐述了VEGF在软骨内成骨、膜内成骨过程中所起的促进作用 ,对成骨细胞和破骨细胞的积极影响 ,增强其表达的相关条件 ,以及各应用方式的利弊 ;从而展示了VEGF在骨缺损修复中的良好的前景。     

血管内皮细胞生长因子及临床应用策略

血管内皮细胞生长因子（VEGF）是一种特异作用于血管内皮细胞的多功能细胞因子,它能引起血管通透性增加,引起细胞外基质成分改变,诱导血管形成,在炎症,创伤愈合,心脏缺血,动脉粥亲硬化,糖尿病性视网膜病变及肿瘤形成等与血管生成和病变有关的诸多病理过程中起重要作用。     

血管内皮细胞生长因子复性条件研究

利用大肠杆菌 BL2 1 (DE3)表达血管内皮细胞生长因子 (VEGF16 5)表达蛋白以包含体形式存在。为了获得有生物活性的蛋白质 ,我们对影响复性的参数 :氧化型、还原型谷胱甘肽比例 ,复性液的 p H值 ,复性时间 ,精氨酸浓度 ,血管内皮细胞生长因子起始浓度进行了较为系统的研究 ,初步获得了具有一定生物活性的 VEGF16 5二聚体蛋白。     

血管内皮生长因子基因治疗大鼠脑缺血的实验研究

为探讨血管内皮生长因子(VEGF)基因治疗大鼠脑缺血的可行性,构建了pcD2/hVEGF121真核表达质粒,建立持续性大脑中动脉堵塞(MCAO)的局灶性脑梗塞模型,大鼠脑皮质直接注射法转移pcD2/hVEGF121真核表达质粒。应用逆转录聚合酶链反应(RT-PCR)、VEGF免疫组织化学法、脑血管计数及梗塞面积测定等方法检测转移pcD2/hVEGF121真核表达质粒后大鼠脑中VEGF基因表达及生物学效应。结果发现,与转移空载质粒的对照组相比,转移VEGF基因后7d的大鼠脑组织中有VEGFmRNA高表达,VEGF免疫组化染色可见VEGF蛋白表达水平增高,脑血管数增多,梗塞体积缩小。因此,直接注射法转移VEGF基因能够在缺血脑组织中表达,表达产物能够发挥生物学效应,进而起到保护脑组织作用。     

血管内皮细胞生长因子与心血管缺血性疾病的治疗

血管内皮细胞生长因子是一种高特异性的促血管内皮细胞生长的因子。由于ＶＥＧＦ在循环中的半衰期短暂,它的基因治将是研究方向。     

血管内皮细胞生长因子及其相关蛋白的结构与功能

血管内皮细胞生长因子（ＶＥＧＦ）是在胚胎发生和创伤愈合过程中启动血管形成的一个高度特异的有丝分裂原,也是一种有效的血管通透性诱导因子,ＶＥＧＦ是胱氨酸结生长因子超家族的一员,它与其受体的结构细节和工能特征为设计分子拮抗剂提供了重要依据。其结构特征和生物学特性使之在缺血组织重组侧支循环,肿瘤预后,肿瘤转移乃至实施基因治疗等领域成为重要的研究对象。     

血管内皮细胞生长因子及其受体的分子生物学研究进展

血管内皮细胞生长因子（ｖａｓｃｕｌａｒ ｅｅｎｄｏｔｈｅｌｉａｌ ｃｅｌｌ ｇｒｏｗｔｈ ｆａｃｔｏｒ,ＶＥＧＦ）是最直接的血管内皮细胞促分裂素,它通过其受体（ＶＥＧＦＲ）介导其活性,不同ＶＥＧＦ剪接体与不同类型的ＶＥＧＦＲ结合,通过胞内信号传导,发挥不同的生物学效应。本总结了ＶＥＧＦ及其受体的结构、特点、分类、分子生物学特征、二的连续及由ＶＥＧＦ诱导的胞内信号传导作用,并简单讨论了它们可能的     

内质网应激条件下血管内皮细胞生长因子在人脑微血管内皮细胞中的表达

为观察内质网应激条件下血管内皮细胞生长因子的表达情况,用不同浓度的衣霉素处理体外培养的人脑微血管内皮细胞,建立内质网应激模型,采用RT—PCR、蛋白质免疫印迹以及免疫细胞化学的方法检测了细胞内血管内皮细胞生长因子的表达。结果发现血管内皮细胞生长因子在人脑微血管内皮细胞中存在一定的表达;内质网应激可诱导血管内皮细胞生长因子表达升高,随着衣霉素浓度的增高,血管内皮细胞生长因子的表达逐渐增加,与mRNA水平相比,血管内皮细胞生长因子蛋白量的增加更明显。实验结果提示人脑微血管内皮细胞中存在血管内皮细胞生长因子自分泌,血管内皮细胞生长因子可能是内质网应激的靶基因。     

VEGF 164 gene transfer by electroporation improves diabetic sensory neuropathy in mice

BACKGROUND: Diabetic neuropathy is the most common cause of peripheral neuropathy and a serious complication of diabetes. Vascular endothelial growth factor (VEGF) stimulates angiogenesis and has neurotrophic and neuroprotective activities. To examine the efficiency of VEGF 164 electro-gene therapy for neuropathy, intramuscular VEGF 164 gene transfer by electroporation was performed to treat sensory neuropathy in diabetic mice. METHODS: VEGF 164 was overexpressed in the tibial anterior (TA) muscles of streptozotocin-induced diabetic mice with hypoalgesia, using a VEGF 164 plasmid injection with electroporation. From 2 weeks after electro-gene transfer, the nociceptive threshold was measured weekly using the paw-pressure test. The TA muscles, sciatic nerve, liver and spleen were histochemically examined at 4 weeks after electro-gene transfer. RESULTS: Two weeks after electro-gene transfer into the bilateral TA muscles, the elevated nociceptive threshold was decreased to a normal level in all treated mice. Improvement of the hypoalgesia continued for 14 weeks. When the VEGF 164 plasmid was injected with electroporation into a unilateral TA muscle, recovery from hypoalgesia was observed in not only the ipsilateral hindpaw, but also the contralateral one, suggesting that VEGF circulates in the blood. No increase in the number of endoneurial vessels in the sciatic nerve was found in the VEGF 164 plasmid-electroporated mice. CONCLUSIONS: These findings suggest that VEGF 164 electro-gene therapy completely recovered the sensory deficits, i.e. hypoalgesia, in the diabetic mice through mechanisms other than angiogenesis in the endoneurium of the peripheral nerve, and may be useful for treatment for diabetic sensory neuropathy in human subjects.     

血管内皮生长因子受体的结构与功能

血管内皮生长因子(VEGF)受体是存在于血管内皮细胞,介导内皮细胞增殖分化的跨膜受体.研究较多的有两种VEGF特异受体:Flt和KDR.Flt和KDR的基因结构及染色体定位已基本确定,这二者均属RTK Ⅲ型受体,结构相似.细胞外区均有7个类似免疫球蛋白结构,细胞内区催化域均有酪氨酸激酶插入区.当VEGF与受体结合时,引起受体自身的磷酸化,发生细胞内反应.在血管发生与生长、创伤修复、炎症、肿瘤和某些血管疾病中起重要作用.     

VEGF受体功能研究进展

血管内皮生长因子受体（VEGFR）调控心血管系统的发育。VEGFR1对于造血祖细胞的招募及单核巨噬细胞的迁移是必需的;VEGFR2、VEGFR3在调控血管及淋巴管内皮细胞的功能时发挥重要作用,而现在很多研究都聚焦于阻断VEGFR信号通路以达到阻断肿瘤血管生长的目的。     

缺氧条件下血管活性因子对血管内皮细胞中VEGF表达的影响

 探讨在缺氧条件下人脐静脉血管内皮细胞对血管内皮生长因子 (vascular endothelialgrowth factor,VEGF)表达及缩血管活性物质内皮素 (ET)、舒血管活性物质一氧化氮 (NO)和 NO抑制剂 LNNA对 VEGF基因表达的影响 .体外培养人脐静脉血管内皮细胞 ,经缺氧及血管活性物质处理 .Northern杂交、酶联免疫检测和计算机图象分析等观察 VEGF m RNA和蛋白表达水平 .发现缺氧 6h内皮细胞可见 VEGF表达 .ET可促进 VEGF m RNA的表达 ,NO可明显抑制 VEGFm RNA的表达 ,NO抑制剂 LNNA也影响 VEGF m RNA的表达 .ELISA检测 VEGF蛋白水平分别为 6h组 8.2± 1 .1 ng/ L,ET+6h组 9.37± 1 .0 2 ng/ L,NO+6h组 2 .86± 0 .91 ng/ L,L - NNA+6h组 1 4.75± 1 .87ng/ L.缺氧可诱导人脐静脉血管内皮细胞分泌 VEGF并受血管活性物质ET和 NO的调控 ,ET促进其表达 ,NO抑制其表达 .     

阻断VEGF旁分泌通路抑制乳腺癌血管生成与肿瘤生长

以人乳腺癌细胞株MCF 7为研究对象 ,通过构建有义与反义血管内皮生长因子 (VEGF)基因表达质粒 ,并转染MCF 7细胞 ,建立了高与低水平表达VEGF的细胞克隆。稳定转染反义VEGF表达质粒的细胞产生和分泌VEGF的能力明显下降 ,尽管在体外培养条件下细胞的增殖速度与未经转染的对照相比不是减慢而是略有增快 ,但在体内的成瘤能力、生长速度和转移能力等却明显低于未经转染的对照细胞或稳定转染有义VEGF表达质粒高水平表达VEGF的细胞克隆。通过体内电穿孔技术介导反义VEGF12 1及可溶性VEGF受体sFlk 1表达质粒转移至荷瘤鼠肿瘤组织内 ,反义VEGF12 1及sFlk 1的表达能显著抑制肿瘤的生长。研究结果证实了VEGF旁分泌通路在诱导乳腺癌肿瘤血管生成、促进肿瘤生长和转移方面起重要作用 ,阻断VEGF旁分泌通路能有效抑制乳腺癌的生长     

靶向抑制VEGF在肺癌治疗中的应用前景

血管内皮生长因子（vascular endothelial growth factor,VEGF）是介导肿瘤血管生成最重要因子,与肺癌细胞增殖、转移及预后密切相关。靶向沉默VEGF基因及抑制其受体表达在肺癌治疗中具有光明的应用前景。本文就此进行综述。     

Screening of human vascular endothelial growth factor (VEGF) receptor Flt-1 domain and study on its biological activity

Four human vascular endothelial growth factor receptor Flt-1 cDNA fragments containing extracellular domain loops 2, 1–2, 2–3 and 1–3 respectively were amplified from human placental cDNA library by PCR and used for screening ligand binding domains by yeast two-hybrid system. The result showed that, not only loop 1–3, but also the smaller fragment loop 2–3 could bind to hVEGF₁₆₅. Recombinant expression plasmids pPIC9K/Flt-1(1–3) and pPIC9K/Flt-1(2–3) were constructed and transformed toPichia. pastoris host strain GS115, cultured in flasks, and expressed under the induction of 1% methanol. The expressed product existed in supernatant in the form of soluble molecules and contained more than 60% of total protein after being induced for 4d. After being purified by CM-Sepharose FF and Sephacryl S-100 chromatography, its purity reached above 90%. Biological assayin vitro showed that the binding capacity of expressed soluble Flt-1 (2–3) to hVEGF₁₆₅ and its inhibiting effect on the proliferation of human umbilical veins endothelial cells (HUVEC) stimulated with hVEGF₁₆₅ were close to those of sFlt-1(1–3). Animal test showed that sFlt-1(2–3) could inhibit the formation of regenerate blood vessels stimulated with hVEGF₁₆₅ significantly.     

FACS-purified myoblasts producing controlled VEGF levels induce safe and stable angiogenesis in chronic hind limb ischemia

We recently developed a method to control the in vivo distribution of vascular endothelial growth factor (VEGF) by high throughput Fluorescence-Activated Cell Sorting (FACS) purification of transduced progenitors such that they homogeneously express specific VEGF levels. Here we investigated the long-term safety of this method in chronic hind limb ischemia in nude rats. Primary myoblasts were transduced to co-express rat VEGF-A(164) (rVEGF) and truncated ratCD8a, the latter serving as a FACS-quantifiable surface marker. Based on the CD8 fluorescence of a reference clonal population, which expressed the desired VEGF level, cells producing similar VEGF levels were sorted from the primary population, which contained cells with very heterogeneous VEGF levels. One week after ischemia induction, 12 × 10(6) cells were implanted in the thigh muscles. Unsorted myoblasts caused angioma-like structures, whereas purified cells only induced normal capillaries that were stable after 3 months. Vessel density was doubled in engrafted areas, but only approximately 0.1% of muscle volume showed cell engraftment, explaining why no increase in total blood flow was observed. In conclusion, the use of FACS-purified myoblasts granted the cell-by-cell control of VEGF expression levels, which ensured long-term safety in a model of chronic ischemia. Based on these results, the total number of implanted cells required to achieve efficacy will need to be determined before a clinical application.