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[抗狂犬病病毒磷蛋白多克隆抗体的制备与鉴定]

[Production and characterization of a polyclonal antibody against rabies virus phosphoprotein].

作者信息

Castañeda Nadia Yadira, Chaparro-Olaya Jacqueline, Castellanos Jaime E

机构信息

Instituto de Virología, Universidad El Bosque, Bogotá, D. C, Colombia.

出版信息

Biomedica. 2007 Jun;27(2):257-67. Epub 2007 Aug 21.

PMID:17713636
Abstract

INTRODUCTION

The expression of recombinant viral proteins has been a useful tool to study molecular biology and pathogenesis of virus infections. Because commercial specific antibodies to rabies virus phosphoprotein (P) are currently unavailable, these antibodies must be generated de novo in order to study the role of P protein during the infectious process.

OBJECTIVE

A polyclonal antibody was produced and characterized for use against the phosphoprotein (P) of rabies virus. The antibody was raised in rabbits with a recombinant viral phosphoprotein (P) produced in Escherichia coli.

MATERIALS AND METHODS

Gene P coding for the viral phosphoprotein (P) was amplified by RT-PCR and cloned into the expression vector PinPoint Xa-1 T. The recombinant protein P was expressed in Escherichia coli, purified by affinity chromatography and used to produce a polyclonal antibody anti-P. The antibody anti-P was purified and characterized by immunocytochemistry, immunofluorescence, fluorometric CELL-ELISA and Western blotting.

RESULTS

The recombinant viral phosphoprotein was successfully expressed as a 50 kd biotinylated fusion protein which corresponds to the whole protein P of rabies virus. The polyclonal antibody raised against this recombinant protein P was able to detect with high specificity, protein P in cultures of sensorial neurons infected with rabies virus.

CONCLUSIONS

The P protein obtained from heterologous expression in Escherichia coli became a specific antigen that was used to produce a polyclonal antibody capable of detecting native P protein in rabies virus infected cells.

摘要

引言

重组病毒蛋白的表达一直是研究病毒感染的分子生物学和发病机制的有用工具。由于目前尚无针对狂犬病病毒磷蛋白(P)的商业特异性抗体,因此必须重新制备这些抗体,以便研究P蛋白在感染过程中的作用。

目的

制备并鉴定一种针对狂犬病病毒磷蛋白(P)的多克隆抗体。该抗体是用在大肠杆菌中产生的重组病毒磷蛋白(P)免疫兔子制备的。

材料与方法

通过RT-PCR扩增编码病毒磷蛋白(P)的基因P,并将其克隆到表达载体PinPoint Xa-1 T中。重组蛋白P在大肠杆菌中表达,通过亲和层析纯化,并用于制备抗P多克隆抗体。抗P抗体通过免疫细胞化学、免疫荧光、荧光细胞ELISA和Western印迹进行纯化和鉴定。

结果

重组病毒磷蛋白成功表达为50kd的生物素化融合蛋白,与狂犬病病毒的全长蛋白P相对应。针对该重组蛋白P产生的多克隆抗体能够高度特异性地检测狂犬病病毒感染的感觉神经元培养物中的蛋白P。

结论

从大肠杆菌中异源表达获得的P蛋白成为一种特异性抗原,用于制备能够检测狂犬病病毒感染细胞中天然P蛋白的多克隆抗体。

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