[Construction of RNA-containing virus-like nanoparticles expression vector with cysteine residues on surface and fluorescent decoration].

Yi chuan xue bao = Acta genetica Sinica Pub Date : 2005-08-01

Yang-Jian Cheng, Ji-Xuan Liang, Qing-Ge Li

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Abstract

Site-directed mutagenesis was performed at the codon 15 of the MS2 bacteriophage coat protein gene,which had been cloned to the virus-like particles expression vector containing non-self RNA fragment. The produced expression vector,termed pARSC, was transformed to E. coli DH5alpha. The positive clones were selected and proliferated. The harvested cells were treated with sonication and the supernatant was then subjected to linear sucrose density gradients centrifugation (15% to 60%) at 32000 r/min for 4 h at 4 degrees C. The virus-like particles, VLP-Cy, were collected at 35% sucrose density. The particles were examined by transmission electron microscopy and the spherical viral particles of approximately 27 nm in diameter were found. The thiolated VLP-Cy was then chemically modified with fluorescein -5'-maleimide. The covalent fluorescent labeling was confirmed by absorption analysis, SDS-PAGE and MALDI-TOF mass spectroscopy. This is the first report of preparation of RNA-containing natural fluorescent nanoparticles. The study highlight the versatility of MS2 bacteriophage capsids as building blocks for functional nanomaterials construction for a variety of application purposes.

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[表面有半胱氨酸残基的含rna病毒样纳米颗粒表达载体的构建及荧光修饰]。

将已克隆到含有非自身RNA片段的病毒样颗粒表达载体上的MS2噬菌体外壳蛋白基因密码子15进行定点诱变。将生成的表达载体pARSC转化为大肠杆菌dh5 α。选择阳性克隆进行增殖。将收获的细胞超声处理，然后将上清液在4℃下以线性蔗糖密度梯度(15% ~ 60%)在32000 r/min下离心4 h，在35%蔗糖密度下收集病毒样颗粒VLP-Cy。通过透射电子显微镜对颗粒进行检测，发现直径约为27 nm的球形病毒颗粒。然后用荧光素-5′-马来酰亚胺对巯基化的VLP-Cy进行化学修饰。通过吸收分析、SDS-PAGE和MALDI-TOF质谱分析证实了共价荧光标记。这是首次报道制备含rna的天然荧光纳米颗粒。该研究强调了MS2噬菌体衣壳作为各种应用目的的功能纳米材料构建块的多功能性。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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Yi chuan xue bao = Acta genetica Sinica

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