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Gag-derived proteins of HIV-1 isolates from Indian patients: Cloning, expression, and purification of p24 of B- and C-subtypes

机译:印度患者HIV-1分离株的Gag衍生蛋白:B和C亚型p24的克隆,表达和纯化

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摘要

A simple and efficient method for hyperexpression in Escherichia coli and purification of capsid protein, p24, of human immunodeficiency virus type 1 (HIV-1) of both B- and C-subtypes is described. DNA-encoding p24 of C-subtype was cloned from C-subtype gag sequence which was obtained by PCR amplification using DNA extracted from peripheral blood mononuclear lymphocytes (PBMLs) of an HTV-1-infected patient from India, DNA-encoding p24B protein was amplified directly by two-step PCR using genomic DNA obtained from PBMLs of an PW-infected individual, A T7 promoter-based expression system was optimized for hyperexpression of p24 in the soluble form. Both p24 (B- and C-subtype) were purified to near homogeneity using conventional chromatographic techniques. Purification of p24 (C subtype) was described for the first time with yield of 53 mg from 1 liter of culture. The yield of p24 (B-subtype) was 67 mg from 1 liter of culture, which was severalfold better than reported earlier, The immunoreactivity of both types of p24 to sera from HIV-infected individuals was comparable. This report describes a simple, highly efficient, and reproducible method for obtaining large quantities of highly pure p24 of both B- and C-subtype, which can be used for structural, biochemical, and inmunological characterization and, eventually, for diagnostic and prognostic applications. (C) 2000 Academic Press. [References: 24]
机译:描述了一种简单高效的方法,用于在大肠杆菌中过表达和纯化B型和C型人免疫缺陷病毒1型(HIV-1)的衣壳蛋白p24。从印度感染HTV-1的患者外周血单核淋巴细胞(PBML)中提取的DNA通过PCR扩增从C亚型gag序列中克隆出编码C24亚型的p24B蛋白,该DNA编码p24B蛋白是通过使用从感染PW的个体的PBML获得的基因组DNA通过两步PCR直接扩增,优化了基于T7启动子的表达系统,以可溶性形式过度表达p24。使用常规色谱技术将p24(B和C亚型)纯化至接近均一。首次描述了p24(C亚型)的纯化,从1升培养物中获得53 mg的产量。从1升培养物中得到的p24(B亚型)产量为67 mg,比早先报道的要好几倍。两种类型的p24对HIV感染者血清的免疫反应性相当。本报告介绍了一种简单,高效且可重现的方法,用于获取大量B型和C型亚型的高纯度p24,可用于结构,生化和免疫学表征,并最终用于诊断和预后应用。 (C)2000学术出版社。 [参考:24]

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