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Synthesis, characterization and bio-functionalization of magnetic nanoparticles to improve the diagnosis of tuberculosis

机译:磁性纳米粒子的合成,表征和生物官能化,提高结核病的诊断

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Mycobacterium tuberculosis is the cause of one of the diseases with the highest mortality and morbidity rate in the Americas and in the world. In developing countries, the diagnosis of tuberculosis (TB) is based on baciloscopy and bacteriological cultures. The first method has a low sensitivity, and the second can take several weeks to reach a confirmatory diagnosis. The lack of a rapid diagnosis compromises the efforts to control this disease and favors the transmission of tuberculosis to the susceptible population. In this work, we present the synthesis, amine-silanization, characterization and bio-functionalization of magnetic nanoparticles (MNPs) to develop a sandwich ELISA to detect and concentrate antigens from M. tuberculosis. For this purpose, a recombinant mycobacterial heat shock protein Hsp16.3, which contributes to the persistence of TB, was cloned and expressed in the E. coli system. Polyclonal antibodies anti-Hsp16.3 were produced in a rabbit and in mice. Magnetic nanoparticles were synthesized by coprecipitation, amine-functionalized and characterized by several physical-chemical methods. The XRD, Mossbauer spectroscopy, zeta potential, TEM, and FTIR all proved the successful preparation of the MNPs showing a diffraction crystal diameter of 10.48 +/- 2.56 nm, superficial net charge of.: +23.57 +/- 2.87 mV, characteristic patterns of magnetite and a structure similar to a sphere. Additionally, it showed a magnetization saturation of 37.06 emu.g(-1). For the functionalization of nanoparticle surfaces with anti-Hsp16.3, the active ester method was used for bond formation, and parameters such as time of incubation, coupling agents ratio (EDC/NHS) and concentration as well as surface saturation level of amine-silanized MNPs (MNP@Si@NH2) were standardized. Finally, bio-functionalized MNPs were used to detect, fix and concentrate the recombinant antigen Hsp16.3 from M. tuberculosis in a sandwich ELISA-MNP assay.
机译:结核分枝杆菌是美洲和世界上具有最高的死亡率和发病率最高的疾病的原因。在发展中国家,结核病(TB)的诊断基于释胆术和细菌培养物。第一种方法具有较低的灵敏度,第二个方法可能需要几周才能达到确认诊断。缺乏快速诊断损害了控制这种疾病的努力,并有利于结核病对易感人群的速度传播。在这项工作中,我们介绍了磁性纳米粒子(MNP)的合成,胺 - 硅烷化,表征和生物官能化,以产生夹心ELISA,以检测和浓缩来自M.结核病的抗原。为此目的,克隆并在大肠杆菌系统中克隆并表达了有助于TB的持续性的重组分枝杆菌热休克蛋白HSP16.3。多克隆抗体抗HSP16.3在兔和小鼠中产生。通过共沉淀,胺官能化合成磁性纳米粒子,并通过几种物理化学方法表征。 XRD,Mossbauer光谱,Zeta电位,TEM和FTIR都证明了MNP的成功制备,显示出衍射晶体直径为10.48 +/- 2.56nm,浅表净电荷,+23.57 +/- 2.87 mV,特征模式磁铁矿和类似于球体的结构。另外,它显示出37.06 emu.g(-1)的磁化饱和度。对于抗HSP16.3的纳米粒子表面的官能化,活性酯方法用于键形成,以及孵育时间,偶联剂比(EDC / NHS)和浓度以及胺的表面饱和水平的参数 - 标准化硅烷化MNPS(MNP @ SI @ NH2)。最后,生物官能化的MNP用于检测,固定和浓缩三明治ELISA-MNP测定中的M.结核病的重组抗原Hsp16.3。

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