Zhu Han-Ping, Yao Ping-Ping, Xu Fang, Weng Jing-Qing, Xie Rong-Hui, Lu Qun-Ying, Zhu Zhi-Yong, Yan Jie
Department of Medical Microbiology and Parasitology, College of Medicine, Zhejiang University, Hangzhou 310058, China.
Zhonghua Liu Xing Bing Xue Za Zhi. 2007 Jul;28(7):692-6.
To clone the gene encoding nucleocapsid protein (NP) of hantavirus strain Z10 (HV-Z10), to construct its prokaryotic expression system as well as to establish a rNP-IgM direct capture ELISA based on HRP-labeled recombinant NP (rNP), in order to detect serum samples of patients suffering from hemorrhagic fever with renal syndrome (HFRS) and to evaluate the effects of detection.
Gene encoding NP of strain HV-Z10 was amplified by PCR and then its prokaryotic expression system pET28a-Z10N-E. coli BL21DE3 was constructed, using routine genetic engineering method. SDS-PAGE was applied to measure the expression of rNP and ion-exchange plus Ni-NTA-affinity chromatography was performed to purify the recombinant product. Western blot assay was used to determine the specific immuno-reactivity of rNP while HRP-labeled rNP-IgM direct capture ELISA was established to detect the serum samples from 95 cases of confirmed HFRS patients. The detection effect was compared with that by routine HV-IgM indirect capture ELISA method.
pET28a-Z10N-E. coli BL21DE3 was able to express rNP with high efficiency. The purified rNP only showed a single protein fragment in the gel after SDS-PAGE. HV-IgG could efficiently recognize rNP and hybridize with the recombinant protein. 94.73% (90/95) of HFRS patients' serum samples were positively confirmed by rNP-IgM direct capture ELISA, while a positive rate of 92.63% (88/95) in the same samples was confirmed by HV-IgM indirect capture ELISA. The distributions of A450 values of the serum samples detected by the two IgM capture ELISAs as well as the changes of the A450 mean values from several serum samples with different dilutions were similar.
We successfully constructed a high efficient prokaryotic expression system of NP encoding gene of hantavirus strain HV-Z10. The rNP-IgM direct capture ELISA that established in this study could be used as a new serological test for HFRS diagnosis because of its simplicity, safety, with high sensitivity and specificity.
克隆汉坦病毒Z10株(HV-Z10)核衣壳蛋白(NP)编码基因,构建其原核表达系统,并建立基于辣根过氧化物酶标记重组NP(rNP)的rNP-IgM直接捕获ELISA法,用于检测肾综合征出血热(HFRS)患者血清标本并评估检测效果。
采用常规基因工程方法,通过PCR扩增HV-Z10株NP编码基因,构建原核表达系统pET28a-Z10N-大肠杆菌BL21DE3。应用SDS-PAGE检测rNP表达情况,采用离子交换和Ni-NTA亲和层析法纯化重组产物。用Western blot法测定rNP的特异性免疫反应性,建立HRP标记的rNP-IgM直接捕获ELISA法检测95例确诊HFRS患者血清标本,与常规HV-IgM间接捕获ELISA法检测效果进行比较。
pET28a-Z10N-大肠杆菌BL21DE3能高效表达rNP。纯化后的rNP经SDS-PAGE后在凝胶上仅显示单一蛋白条带。HV-IgG能有效识别rNP并与重组蛋白杂交。rNP-IgM直接捕获ELISA法确诊HFRS患者血清标本阳性率为94.73%(90/95),HV-IgM间接捕获ELISA法确诊同一标本阳性率为92.63%(88/95)。两种IgM捕获ELISA法检测血清标本的A450值分布以及不同稀释度的几份血清标本A450平均值变化相似。
成功构建了汉坦病毒HV-Z10株NP编码基因的高效原核表达系统。本研究建立的rNP-IgM直接捕获ELISA法操作简便、安全,灵敏度和特异性高,可作为HFRS诊断的新型血清学检测方法。
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