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一种抑制乙型肝炎病毒附着于肝细胞的单克隆抗体所识别的前S1表位最小长度的测定。

Determination of the minimal length of preS1 epitope recognized by a monoclonal antibody which inhibits attachment of hepatitis B virus to hepatocytes.

作者信息

Sominskaya I, Pushko P, Dreilina D, Kozlovskaya T, Pumpen P

机构信息

Hepatological Center, Latvian Medical Academy, Riga.

出版信息

Med Microbiol Immunol. 1992;181(4):215-26. doi: 10.1007/BF00215767.

DOI:10.1007/BF00215767
PMID:1279369
Abstract

The minimal amino acid sequence sufficient to be recognized efficiently by virus-attachment inhibiting murine monoclonal anti-preS1 antibody MA18/7 has been determined. We have constructed a recombinant gene library using the cloned coat protein gene of Escherichia coli RNA bacteriophage fr as a carrier. Different fragments of preS1 region from cloned hepatitis B virus (HBV) genomes, subtype ayw and adw, were inserted at position 2 of the 129 amino acid-long fr coat protein gene in the appropriate E. coli expression vectors. Fine mapping of preS1 epitope recognized by MA18/7 was accomplished by bidirectional shortening of the preS1 within original recombinant preS-fr coat protein genes with Bal31 exonuclease. Immunoblot analysis of the obtained recombinant protein library revealed that the tetrapeptide Asp-Pro-Ala-Phe (DPAF), located at the position preS(31-34) and conserved in all known HBV genomes, is sufficient to bind MA18/7 antibody. Recognition of the preS1 region by MA18/7 occurred irrespective of the amino acid context surrounding this DPAF tetrapeptide. Further shortening of this minimal epitope from the left or from the right side completely prevented antibody binding in immunoblots.

摘要

已确定足以被病毒附着抑制性鼠单克隆抗前S1抗体MA18/7有效识别的最小氨基酸序列。我们以大肠杆菌RNA噬菌体fr的克隆外壳蛋白基因作为载体构建了一个重组基因文库。将来自克隆的乙型肝炎病毒(HBV)基因组ayw和adw亚型的前S1区域的不同片段,插入到合适的大肠杆菌表达载体中129个氨基酸长的fr外壳蛋白基因的第2位。通过用Bal31核酸外切酶双向缩短原始重组前S-fr外壳蛋白基因中的前S1,完成了对MA18/7识别的前S1表位的精细定位。对所得重组蛋白文库的免疫印迹分析表明,位于前S(31 - 34)位置且在所有已知HBV基因组中保守的四肽天冬氨酸-脯氨酸-丙氨酸-苯丙氨酸(DPAF)足以结合MA18/7抗体。MA18/7对前S1区域的识别与该DPAF四肽周围的氨基酸背景无关。从左侧或右侧进一步缩短这个最小表位完全阻止了免疫印迹中的抗体结合。

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