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诺氏疟原虫一种与红细胞上达菲抗原配体结合的疟疾蛋白的受体样特异性。

Receptor-like specificity of a Plasmodium knowlesi malarial protein that binds to Duffy antigen ligands on erythrocytes.

作者信息

Haynes J D, Dalton J P, Klotz F W, McGinniss M H, Hadley T J, Hudson D E, Miller L H

机构信息

Department of Immunology, Walter Reed Army Institute of Research, Washington, DC 20307.

出版信息

J Exp Med. 1988 Jun 1;167(6):1873-81. doi: 10.1084/jem.167.6.1873.

Abstract

A 135-kD parasite protein, a minor component of the Plasmodium knowlesi malaria radiolabeled proteins released into culture supernatant at the time of merozoite release and reinvasion, specifically bound to human erythrocytes that are invaded and carry a Duffy blood group determinant (Fya or Fyb), but did not bind to human erythrocytes that are not invaded and do not carry a Duffy determinant (FyFy). Specific anti-Duffy antibodies blocked the binding of the 135-kD protein to erythrocytes carrying that specific Duffy determinant. Purified 135-kD protein bound specifically to the 35-45-kD Duffy glycoprotein on a blot of electrophoretically separated membrane proteins from Fya and Fyb erythrocytes but not from FyFy erythrocytes. Binding of the 135-kD protein was consistently greater to Fyb than to Fya both on the blot and on intact erythrocytes. The 135-kD protein also bound to rhesus erythrocytes that are Fyb and are invaded, but not to rabbit or guinea pig erythrocytes that are Duffy-negative and are not invaded. Cleavage of the Duffy determinant by pretreating Fyb human erythrocytes with chymotrypsin greatly reduced both invasion and binding of the 135-kD protein, whereas pretreating Fyb erythrocytes with trypsin had little effect on the Duffy antigen, the 135-kD protein binding, or on invasion. However, instances of invasion of other enzyme-treated erythrocytes that are Duffy-negative and do not bind the 135-kD protein suggest that alternative pathways for invasion do exist.

摘要

一种135-kD的寄生虫蛋白,是诺氏疟原虫疟疾放射性标记蛋白的次要成分,在裂殖子释放和再侵入时释放到培养上清液中,它特异性地结合到被侵入并携带达菲血型决定簇(Fya或Fyb)的人类红细胞上,但不结合未被侵入且不携带达菲决定簇(FyFy)的人类红细胞。特异性抗达菲抗体可阻断135-kD蛋白与携带该特定达菲决定簇的红细胞的结合。纯化的135-kD蛋白在来自Fya和Fyb红细胞而非FyFy红细胞的电泳分离膜蛋白印迹上,特异性地结合到35 - 45-kD的达菲糖蛋白上。在印迹和完整红细胞上,135-kD蛋白与Fyb的结合始终比与Fya的结合更强。135-kD蛋白也结合到Fyb且被侵入的恒河猴红细胞上,但不结合达菲阴性且未被侵入的兔或豚鼠红细胞。用胰凝乳蛋白酶预处理Fyb人类红细胞以切割达菲决定簇,可大大降低135-kD蛋白的侵入和结合,而用胰蛋白酶预处理Fyb红细胞对达菲抗原、135-kD蛋白结合或侵入几乎没有影响。然而,其他酶处理的达菲阴性且不结合135-kD蛋白的红细胞存在侵入的情况表明,确实存在替代的侵入途径。

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