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Analysis of antigenic domain of GST fused major surface protein (p30) fragments of Toxoplasma gondii

机译:弓形虫GST融合主要表面蛋白(p30)片段的抗原结构域分析

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Antigenic domain of major surface protein (p30) of Toxoplasma gondii was analyzed after polymerase chain reaction (PCR) of its gene fragments. Hydrophilic or hydrophobic moiety of amino acid sequences were expressed as glutathione S-transferase (GST) fusion proteins. Fragments of p30 gene were as follows: T37, total p30 open reading frame (ORF); S28, total ORF excluding N-terminal signal sequence and C- terminal hydrophobic sequence: A19, N-terminal 2/3 parts of S28; P19, C- terminal 2/3 of S28; X9, N-terminal 1/3 part of S28; Y10, middle 1/3 of S28; and Z9, C-terminal 1/3 of S28, respectively. Primer of each fragment was synthesized to include clamp sequence of EcoR I restriction site. PCR amplified DNA was inserted into GST (26 kDa) expression vector, pGEX-4T-1 to transform into Escherichia coli (JM105 strain). GST fusion proteins were expressed with IPTG induction as 63, 54, 45, 45, 35, 36, and 35 kDa proteins measured by SDS-PAGE. Each fusion protein was confirmed with GST detection kit. Western blot analysis with the serum of a toxoplasmosis patient revealed antigenicity in proteins expressed by T37, S28, and A19 but not those by P18, X9, Y10, and Z9. Antigenicity of p30 seems to be located either in N-terminal 1/3 part in the presence of middle 1/3 part or in the oligopeptides between margins of the first and second 1/3 parts.
机译:弓形虫的基因片段的聚合酶链反应(PCR)后,分析了弓形虫主要表面蛋白(p30)的抗原结构域。氨基酸序列的亲水或疏水部分表示为谷胱甘肽S-转移酶(GST)融合蛋白。 p30基因的片段如下:T37,总p30开放阅读框(ORF); S28,不包括N端信号序列和C端疏水序列的总ORF:A19,S28的N端2/3部分; P19,S28的C / 2/3端子; X9,S28的N端1/3; Y10,S28的中间1/3;和Z9,分别是S28的C端1/3。合成每个片段的引物以包括EcoRI限制性位点的钳位序列。将PCR扩增的DNA插入GST(26kDa)表达载体pGEX-4T-1,以转化到大肠杆菌(JM105菌株)中。通过SDS-PAGE测定,GST融合蛋白通过IPTG诱导表达为63、54、45、45、35、36和35 kDa蛋白。用GST检测试剂盒确认每种融合蛋白。用弓形虫病患者血清进行的蛋白质印迹分析显示,T37,S28和A19表达的蛋白质具有抗原性,而P18,X9,Y10和Z9则没有。 p30的抗原性似乎位于中间1/3部分的N末端1/3部分中,或者位于第一和第二个1/3部分的边缘之间的寡肽中。

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