硅纳米颗粒作为基因转染载体的研究

通过不同浓度的NaCl、NaI修饰硅纳米颗粒,用琼脂糖凝胶电泳分析硅纳米颗粒与DNA结合力及对DNA的保护作用,同时用绿色荧光蛋白基因作报告基因,以硅纳米颗粒作为基因转染的载体,转染HT1080细胞。经电镜观察证实硅纳米颗粒进入细胞内;硅纳米颗粒与DNA结合后,能对DNA起保护作用;并且硅颗粒作为基因转染的载体,将绿色荧光蛋白基因导入HT1080细胞,用荧光显微镜观察到发绿色荧光的细胞。结果表明,硅纳米颗粒可作为基因转染的载体。     

磁性纳米颗粒作为载体在基因转染中的研究进展

磁性纳米颗粒具有很强的结合、浓缩与保护DNA的作用,具有超顺磁性、较高的安全性和低的免疫原性,可以结合大片段DNA,在外加磁场的作用下可实现安全、高效的基因靶向性运输,提高外源基因的转染效率。由于磁性纳米颗粒的独特性质,使得其作为非病毒载体在基因治疗中的应用进展迅速。我们简要介绍磁性纳米材料的特点、种类及结构,磁性纳米基因载体的特点,以及磁性纳米颗粒作为载体在基因转染中的应用情况。     

磁性纳米颗粒作为基因转染载体的研究

通过扫描电子显微镜和Zeta电位仪对磁性纳米颗粒的形貌、粒径、表面电位等进行了表征。利用凝胶电泳阻滞试验分析磁性纳米颗粒与DNA的结合情况,研究磁性纳米颗粒对DNA的保护效果,运用MTT和流式细胞术分析磁性纳米颗粒对细胞的毒性。以绿色荧光蛋白基因为报告基因进行293T细胞的转染,研究磁性纳米颗粒与质粒DNA不同比例条件下对293T细胞的转染效率,并与脂质体(Lipofectamine2000)介导的转染进行比较分析。结果表明,磁性纳米颗粒与DNA可以稳定结合,可以保护DNA免受酶的消化作用,当磁性纳米颗粒与DNA比为1 1时,转染效率最高,优于脂质体(Lipotamine2000)介导的转染,且对细胞的毒害作用小于Lipotamine2000。     

磁性纳米颗粒介导基因转染的研究进展

介绍了磁性纳米颗粒介导基因转染的最新研究进展,面临的主要问题以及将来的发展方向。     

涡旋磁纳米颗粒——崭新的生物医用磁性纳米平台

相比于超顺磁性纳米颗粒,具有涡旋磁畴的磁性纳米颗粒,由于独特的磁化闭合分布、较大的粒径尺寸及外加磁场中的磁化翻转特性,使得其兼具弱的颗粒间磁相互作用和更优异的磁学性能,在生物医学领域展现出了更好的应用优势和潜力.本综述结合近年来国内外对涡旋磁畴的研究及涡旋磁纳米颗粒在生物医学领域的报道,提出了一类新型的生物医用涡旋磁溶胶体系,并以涡旋磁氧化铁纳米盘和纳米环为例,介绍了涡旋磁纳米颗粒的化学合成,并着重论述了这类具有独特涡旋畴结构的纳米颗粒在磁共振成像、抗肿瘤治疗等生物医学应用上的最新研究进展.     

微生物介导的金纳米颗粒合成

金纳米颗粒凭借其独特的光学和电化学特性,广泛应用于信息存储、化学传感、医学成像、药物传输以及生物标记等领域。近年来,生物法合成金纳米颗粒因其环境友好、绿色低毒等特点引起研究者的广泛关注。研究表明,多种微生物包括细菌、放线菌、真菌和病毒等均具有合成金纳米颗粒的能力。本文综述了微生物介导合成金纳米颗粒的特性、机制及应用,并对未来发展趋势进行了展望。     

相互作用对纳米颗粒跨生物膜输运的影响

纳米颗粒与生物膜之间的相互作用,对于纳米颗粒在细胞成像、生物传感器设计、药物输送及疾病诊断和治疗等方面的应用有着重要的影响.本文采用自洽场理论,考察了不同相互作用条件下,纳米颗粒跨膜输运过程中生物膜的形变情况,以及系统自由能的变化情况.结果表明,在纳米颗粒跨膜输运的过程中,随着纳米颗粒与生物膜之间相互作用的改变,生物膜...     

聚合物纳米颗粒对动脉粥样硬化病变的影响及相关机理研究进展

聚合物纳米颗粒通常指基于疏水性聚合物的纳米粒子,由于其良好的生物相容性、高效的长循环特性以及优于其他纳米颗粒物的代谢排出方式等,在纳米医学领域中得到了广泛关注。现有研究证明聚合物纳米颗粒在心血管疾病,尤其是在动脉粥样硬化(atherosclerosis,AS)的诊断、治疗中具有独特的优点,已经成功地由基础研究向临床应用转化。但是聚合物纳米颗粒引起的炎症反应诱导泡沫细胞形成、巨噬细胞自噬,以及心血管系统疾病力学微环境改变引起的聚合物纳米颗粒富集等,都可能最终诱导AS的发生发展。在此,本文综述了近年来聚合物纳米颗粒在诊断、治疗AS疾病中的应用及其与AS病变的关系和机理,为后续研究利用聚合物纳米颗粒开发新型纳米药物治疗AS提供理论依据。     

利用纳米技术转运药物

将纳米技术引入药物转运系统，不只是关于显微颗粒．的话题。Cytlmmune Sciences公司首席执行官及创立人之一的LarryTamarkin说：“我把纳米药物看作全新的药物实体。”此技术的发展，基于纳米级颗粒、特定药物与疾病的生物与化学知识。     

纳米颗粒和蛋白质：何其相似耶？

纳米颗粒,即尺寸为纳米级（一般在1-100 nm之间）,处在原子簇和微尺度物体过渡区域内的粒子,又称超微颗粒,一般都是人工合成的产物。蛋白质是人类生命活动最重要的物质基础,是构成一切细胞和组织结构必不可少的成分,但从本质上出发,它是一类具有生物活性的有机生物高分子。两者看似属于不同的科学范畴,但是近十年来的研究发现,纳米颗粒和蛋白质在很多方面具有惊人的相似,例如尺寸、结构、电荷、表面化学组成、分子间相互作用力等。本文将通过一些实例,从不同角度阐述纳米颗粒和蛋白质之间的异同及相互联系。     

Spatio-temporal modeling of nanoparticle delivery to multicellular tumor spheroids

The inefficiency of nanoparticle penetration in tissues limits the therapeutic efficacy of such formulations for cancer applications. Recent work has indicated that modulation of tissue architecture with enzymes such as collagenase significantly increases macromolecule delivery. In this study we developed a mathematical model of nanoparticle penetration into multicellular spheroids that accounts for radially dependent changes in tumor architecture, as represented by the volume fraction of tissue accessible to nanoparticle diffusion. Parameters such as nanoparticle binding, internalization rate constants, and accessible volume fraction were determined experimentally. Unknown parameters of nanoparticle binding sites per cell in the spheroid and pore shape factor were determined by fitting to experimental data. The model was correlated with experimental studies of the penetration of 40 nm nanoparticles in SiHa multicellular spheroids with and without collagenase treatment and was able to accurately predict concentration profiles of nanoparticles within spheroids. The model was also used to investigate the effects of nanoparticle size. This model contributes toward the understanding of the role of tumor architecture on nanoparticle delivery efficiency.     

转铁蛋白修饰磁性纳米粒的制备及其体外抗肿瘤活性研究

目的:本研究旨在构建一种转铁蛋白修饰负载阿霉素(DOX)的磁纳米粒靶向递药系统,以提高阿霉素作用的靶向性。方法:采用化学共沉淀法制备转铁蛋白修饰负载阿霉素的磁性纳米粒(DOX@MNP),采用zeta电位及纳米粒度分析仪测定DOX@MNP的粒径及其zeta电位,透析法评价DOX@MNP的体外释药特征。通过MTT实验,研究DOX@MNP与游离DOX对A549细胞的细胞毒性,通过激光共聚焦显微镜和流式细胞仪观察A549细胞对DOX@MNP与游离DOX的摄取情况。结果:DOX@MNP的释药具有p H依赖性。MTT实验结果显示,DOX@MNP与游离DOX具有相当的细胞毒性;激光共聚焦显微镜和流式细胞仪检测结果显示A549细胞对DOX和DOX@MNP的摄取没有明显差异。结论:本文构建了一种转铁蛋白修饰包载阿霉素的磁纳米粒,体外结果显示其具有与游离DOX相当的细胞毒性,为进一步进行体内实验奠定了基础。     

Effect of gold nanoparticle on the microscopic morphology of white blood cell

Background:  In medicine, there is limited knowledge on the toxicity of nanoparticles. In medicine, there has been limited knowledge on the effect of nanoparticles on the white blood cell.
Objective:  To evaluate the effect of gold nanoparticle on the microscopic morphology of white blood cell.
Setting:  Chulalongkorn Univesity, Bangkok, Thailand.
Method:  This study was performed as an experimental study. Mixture of gold nanoparticle solution and blood sample was prepared and analysed.
Result:  This work revealed that after mixing the blood sample with gold nanoparticle solution, accumulation of gold nanoparticle in the white blood cell was observed.
Conclusion:  The effect of gold nanoparticle on the white blood cell can be detected and this knowledge can be used in cytotoxic drug treatment.     

磁性纳米技术在癌症基因治疗中的应用

癌症基因组的最新进展使直接针对癌症基因进行治疗具有极大的可能性。然而,需要新的基因传递方法使这种潜力向临床应用转化,为治疗病人服务。磁性纳米技术是通过外部磁场选择性地高效传递治疗基因,还能同时用影像监测体内的传递过程。相比传统的基因传递方法,这种技术能明显提高人类移植肿瘤和不同的内脏器官如肝、肾及中枢神经系统的基因传递效率。因此,磁性纳米技术使活体内癌症的基因治疗进入到新的前沿领域。     

Chemical and biological conjugation strategies for the development of multivalent protein vaccine nanoparticles

The development of subunit vaccine platforms has been of considerable interest due to their good safety profile and ability to be adapted to new antigens, compared to other vaccine typess. Nevertheless, subunit vaccines often lack sufficient immunogenicity to fully protect against infectious diseases. A wide variety of subunit vaccines have been developed to enhance antigen immunogenicity by increasing antigen multivalency, as well as stability and delivery properties, via presentation of antigens on protein nanoparticles. Increasing multivalency can be an effective approach to provide a potent humoral immune response by more strongly engaging and clustering B cell receptors (BCRs) to induce activation, as well as increased uptake by antigen presenting cells and their subsequent T cell activation. Proper orientation of antigen on protein nanoparticles is also considered a crucial factor for enhanced BCR engagement and subsequent immune responses. Therefore, various strategies have been reported to decorate highly repetitive surfaces of protein nanoparticle scaffolds with multiple copies of antigens, arrange antigens in proper orientation, or combinations thereof. In this review, we describe different chemical bioconjugation methods, approaches for genetic fusion of recombinant antigens, biological affinity tags, and enzymatic conjugation methods to effectively present antigens on the surface of protein nanoparticle vaccine scaffolds.     

抗体和寡核苷酸双标记纳米金生物探针的制备及性能分析

基于纳米金粒子与抗体静电吸附作用,与硫醇修饰的寡核苷酸共价结合,建立一种新的双标记纳米金生物探针的制备方法.通过透射电镜（TEM）、紫外光谱、斑点免疫金渗滤法、免疫金银染色光镜观察法、荧光标记法等检测探针表征,及表面抗体活性情况和寡核苷酸的覆盖率,同时采用变性聚丙烯酰胺凝胶电泳（PAGE）检测寡核苷酸的存在.结果表明,纳米金粒子同时连接抗体和寡核苷酸后生物性能良好,且每个纳米金粒子（10±3）nm表面可覆盖寡核苷酸(92±20)条,双标记纳米金生物探针的制备具有简捷、稳定的特点.可作为一种新型探针应用于超微量蛋白质检测.     

Modulation of phytoremediation and plant growth by the treatment with PGPR,Ag nanoparticle and untreated municipal wastewater

The present attempt was made to determine the effects of untreated municipal wastewater (MW) on growth and physiology of maize and to evaluate the role of Ag nanoparticle and plant-growth-promoting rhizobacteria (PGPR) when interacting with MW used for irrigation. It was used for the isolation of PGPR. The isolates were identified and characterized based on the colony morphology, C/N source utilization pattern using miniaturized identification system (QTS 24), catalase (CAT) and oxidase tests, and 16S rRNA sequence analyses. The three PGPR isolates were Planomicrobium chinense (accession no. NR042259), Bacillus cereus (accession no. CP003187) and Pseudomonas fluorescens (accession no. GU198110). The isolates solubilized phosphate and exhibited antibacterial activities against pathogenic bacteria i.e., Staphylococcus aureus, Pseudomonas aeruginosa, Bacillus subtilis, Klebsiella pneumoniae and Escherichia coli and antifungal activities against Helminthosporium sativum and Fusarium solani. The untreated MW irrigation as well as Ag nanoparticle treatment resulted in significant accumulation of Ni in the rhizosphere soil. PGPR induced accumulation of Ni and Pb in the rhizosphere soil and maize shoot. Ag nanoparticle also caused Ni and Pb accumulation in maize shoot. Combined treatment with PGPR, Ag nanoparticle and MW resulted in decreased accumulation of Pb and Ni both in the rhizosphere soil and maize shoot. Combined treatment of Ag nanoparticle, MW and PGPR decreased Na accumulation and increased K accumulation. Ag nanoparticle increased Fe and Co accumulation but decreased Zn and Cu accumulation in MW treatment; in combined treatment, it reduced PGPR-induced accumulation of Co and Fe in the rhizosphere and Co accumulation in shoot. PGPR significantly increased root weight, shoot weight, root length, shoot length, leaf area, and proline, chlorophyll and carotenoid content of the maize plant. Ag nanoparticle also enhanced the leaf area, fresh weight, root length and antioxidant activities of maize. Treatment with Ag nanoparticle increased the gibberellic acid (GA) and abscisic acid (ABA) content of maize leaves but decreased the accumulation of GA in the presence of PGPR and MW.     

Discovery of a sugar-based nanoparticle universally existing in boiling herbal water extracts and their immunostimulant effect

Herbal medicine is mainly prepared from boiling herbal water extracts. Many epoch-making immunosuppressant drugs, such as glycyrrhizic acid (old example) and FTY720 (current example), were developed from herbal secondary metabolites in the boiling water extract by partition with organic solvents. However, few immunostimulants have been discovered by this method. Instead of the usual method, we aimed to find a novel immunostimulant component by two unique methods in the research of herbal medicine: ultracentrifugation and electron microscopy. The immunostimulant was not a secondary metabolite, as expected, but the structure was a nanoparticle formed by a polysaccharide. In addition, we clarified the immune effect of the nanoparticle. Intake of the nanoparticle by phagocytosis resulted in immunostimulant effects by increasing the genes and proteins of inflammatory cytokines in macrophage cells. The immunostimulant effects were inhibited by a phagocytosis inhibitor, cytochalasin D. To the best of our knowledge, this study is the first to describe the discovery of a nanoparticle in boiling herbal water extracts and its immunostimulant properties. This study will provide additional understanding of the efficacy of herbal medicine, in that the immunostimulant nanoparticle universally exists in boiling herbal water extracts. Thus, traditional herbal medicine may be an oldest known nanomedicine. Furthermore, this study suggests that the immunostimulant nanoparticle simply can be obtained from herbal medicine only by ultracentrifugation. We hope that this simple strategy will substantially contribute to drug development, including vaccine adjuvant, in the future.     

Gold‐silver and silver‐silver nanoparticle constructs based on DNA hybridization of thiol‐ and amino‐functionalized oligonucleotides

Metal nanoparticle constructs of particles of different sizes and materials were prepared, using DNA as connecting element. Therefore, gold and silver nanoparticles were functionalized with complementary DNA sequences that enabled a controlled coupling. The well‐established system based on thiolated DNA was thereby complemented with amino‐functionalized DNA. The realization of specific DNA‐DNA bonds due to hybridization was controlled by the ionic strength. The results demonstrate the potential of the combination of different particle sizes, composition as well as coupling chemistry in order to realize controlled conjugates of nanoparticles. (© 2008 WILEY‐VCH Verlag GmbH & Co. KGaA, Weinheim)     

Nanoparticle interactions with blood proteins and what it means: a tutorial review

Nanoparticles find many uses in medicine and biomedical technology. Such applications imply that they must be colloidally stable and do not interact with proteins in the blood or blood serum. A nanoparticle put into the blood will instantaneously be covered by a protein corona that compromises the function of the nanoparticle core, changes the effective size of the nanoparticle, and determines its biological fate. Strategies developed to gain control over nanoparticles in biological fluids, particular in blood, heavily rely on creating a hydrated polymer shell that sterically and osmotically prevents a protein corona from forming. In this tutorial review, we provide an overview of factors that affect the formation of the protein corona in blood and how to prevent it forming. We focus on describing the latest advances in our understanding of how small core-shell nanoparticles (core diameter 4-20 nm in diameter) with a shell of densely grafted polymer chains, a so-called polymer brush, interact with proteins and cells in vitro. Such nanoparticles are among the most well-defined and well-characterized colloids used for biomedical applications, from which an improved understanding of how nanoparticle architecture influences their biological fate can be obtained in detail.