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补体成分C3b直接结合单纯疱疹病毒1型和2型的纯化糖蛋白C。

Complement component C3b binds directly to purified glycoprotein C of herpes simplex virus types 1 and 2.

作者信息

Eisenberg R J, Ponce de Leon M, Friedman H M, Fries L F, Frank M M, Hastings J C, Cohen G H

机构信息

Department of Pathobiology, School of Veterinary Medicine, University of Pennsylvania, Philadelphia 19104.

出版信息

Microb Pathog. 1987 Dec;3(6):423-35. doi: 10.1016/0882-4010(87)90012-x.

DOI:10.1016/0882-4010(87)90012-x
PMID:2849025
Abstract

Cells infected with herpes simplex virus type 1 (HSV-1), but not HSV-2, express on their surfaces a receptor for the complement component C3b. Receptor activity is markedly enhanced by treatment of the infected cells with neuraminidase. Employing a direct binding assay, consisting of purified HSV glycoproteins immobilized on nitrocellulose and iodinated C3b as a probe, we found that C3b binds directly to gC-1, as well as to gC-2, but not to gB or gD from either serotype. C3b binding was enhanced by treatment of gC-1 or gC-2 with neuraminidase. Endo F or endo H treatment of gC-1 had no effect on C3b binding. However, treatment of gC-2 with these endoglycosidases had a marked negative effect on C3b binding. These results suggest that N-linked oligosaccharides are involved in binding of C3b to gC-2, but not gC-1. Alternatively, removal of N-linked oligosaccharides from gC-2 might adversely affect polypeptide conformation. Glycoprotein C-2 also differs from gC-1 in its effects on the complement cascade. Whereas gC-1 accelerated the decay of the alternative pathway C3 convertase and impaired the efficiency of lysis by the components C5 through C9, gC-2 stabilized the active C3 convertase and had little effect on the late-acting components. The dissimilarity of gC-1 and gC-2 with regard to their effects on the complement cascade may have implications regarding the role of these glycoproteins in confronting the host immune response.

摘要

感染1型单纯疱疹病毒(HSV-1)而非2型单纯疱疹病毒(HSV-2)的细胞,其表面表达补体成分C3b的受体。用神经氨酸酶处理感染细胞可显著增强受体活性。采用一种直接结合试验,即将纯化的HSV糖蛋白固定在硝酸纤维素上,并用碘化C3b作为探针,我们发现C3b直接与gC-1以及gC-2结合,但不与任何一种血清型的gB或gD结合。用神经氨酸酶处理gC-1或gC-2可增强C3b的结合。用内切糖苷酶F或内切糖苷酶H处理gC-1对C3b结合没有影响。然而,用这些内切糖苷酶处理gC-2对C3b结合有显著的负面影响。这些结果表明,N-连接寡糖参与C3b与gC-2的结合,但不参与与gC-1的结合。或者,从gC-2上去除N-连接寡糖可能会对多肽构象产生不利影响。糖蛋白C-2在对补体级联反应的影响方面也与gC-1不同。gC-1加速替代途径C3转化酶的衰变,并损害C5至C9成分的裂解效率,而gC-2则稳定活性C3转化酶,对后期作用成分影响很小。gC-1和gC-2在对补体级联反应的影响方面的差异,可能与这些糖蛋白在应对宿主免疫反应中的作用有关。

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