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B:2亚属腺病毒纤维上的表位和血凝结合域。

Epitopes and hemagglutination binding domain on subgenus B:2 adenovirus fibers.

作者信息

Mei Y F, Wadell G

机构信息

Department of Virology, Umeå University, Sweden.

出版信息

J Virol. 1996 Jun;70(6):3688-97. doi: 10.1128/JVI.70.6.3688-3697.1996.

Abstract

The adenovirus fiber serves as a ligand between the virus and the host cell receptor and manifests hemagglutination (HA) activity and antigenic domains. We have screened both the antigenic and immunogenic epitopes on the adenovirus fibers of subgenus B:2 by using recombinant fiber proteins (rfibers) expressed in Escherichia coli, synthesized peptides (P1 to P8), and the corresponding antisera. The results indicated that P4 (amino acids [aa] 201 to 220), P5 (aa 231 to 250), and P7 (aa 275 to 295) presented both antigenic and immunogenic epitopes in adenovirus type 11 prototype (Ad11p), Ad34a, and Ad11a fibers. P6 (aa 251 to 270) presented both epitopes in Ad11a fiber but only an antigenic epitope in other fibers. The C-terminal 20 amino acids of the fiber, corresponding to P8, manifested an epitope of low-level immunogenicity. P5, localized at the N-terminal aa 231 to 250, displayed an epitope that reacted with fibers of all the members of subgenus B analyzed. The rfibers of Ad11p and Ad34a displayed HA activity with monkey erythrocytes, though those of Ad11a did not. Mutagenesis of the rfibers revealed that neither the fragment replacements, 11p20211a, llp26011a,and 11a28011p, nor the Ad11p rfiber with the substitutions of Tyr-260-->H (Tyr260H)and Arg279Q displayed HA activity. The Ad11a fiber knob was sensitive to proteolytic digestion, whereas that of Ad11p was resistant. The results demonstrated that the decisive HA binding domain was presented at aa 260 to 280 and was conformation dependent. Nearby amino acids, aa 283 and 284, may also affect the HA function.

摘要

腺病毒纤维作为病毒与宿主细胞受体之间的配体,具有血凝(HA)活性和抗原结构域。我们利用在大肠杆菌中表达的重组纤维蛋白(rfibers)、合成肽(P1至P8)及相应抗血清,筛选了B亚属2型腺病毒纤维上的抗原表位和免疫原性表位。结果表明,P4(氨基酸[aa]201至220)、P5(aa231至250)和P7(aa275至295)在11型腺病毒原型(Ad11p)、Ad34a和Ad11a纤维中均呈现抗原表位和免疫原性表位。P6(aa251至270)在Ad11a纤维中呈现两种表位,但在其他纤维中仅呈现抗原表位。纤维的C末端20个氨基酸(对应于P8)表现出低水平免疫原性的表位。位于N末端aa231至250的P5呈现出一个与所分析的B亚属所有成员的纤维发生反应的表位。Ad11p和Ad34a的rfibers对猴红细胞表现出血凝活性,而Ad11a的rfibers则没有。rfibers的诱变显示,片段替换11p20211a、llp26011a和11a28011p,以及用Tyr-260→H(Tyr260H)和Arg279Q替换的Ad11p rfiber均未表现出血凝活性。Ad11a纤维钮对蛋白水解消化敏感,而Ad11p的则具有抗性。结果表明,决定性HA结合结构域位于aa260至280,且依赖于构象。附近的氨基酸aa283和284也可能影响HA功能。

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