Purification and analysis of a polydnavirus gene product expressed using a poly-histidine baculovirus vector

被引：17

作者：

Soldevila, AI ^{[1
]}

Heuston, S ^{[1
]}

Webb, BA ^{[1
]}

机构：

[1] UNIV KENTUCKY, DEPT ENTOMOL, LEXINGTON, KY 40546 USA

来源：

INSECT BIOCHEMISTRY AND MOLECULAR BIOLOGY | 1997年 / 27卷 / 03期

关键词：

cysteine-rich; Campoletis sonorensis; Heliothis virescens; Autographa californica; nucleopolyhedrovirus; glycosylation; poly-histidine;

D O I：

10.1016/S0965-1748(96)00087-2

中图分类号：

Q5 [生物化学]; Q7 [分子生物学];

学科分类号：

071010 ; 081704 ;

摘要：

The VHv1.1 polydnavirus gene has been implicated in suppressing the encapsulation response in parasitized insects [Li and Webb (1994) J, Virol. 68, 7482-7489]. In order to characterize this gene product and to further our analysis of its immunosuppressive function, we expressed the VHv1.1 using a custom-designed C-terminal poly-histidine baculovirus vector which allows for high expression and single-step purification of the protein, The 34 kDa VHv1.1 protein was expressed in baculovirus-infected cell cultures and in H. virescens larvae. Highly enriched preparations of the secreted VHv1.1 protein were obtained after affinity chromatography using a NTA-(Ni2+) resin, Characterization with purified preparations of the VHv1.1 protein established that the protein is N-glycosylated, containing glycogroups which are PNGase F-sensitive but Endo H-resistant. The recombinant VHv1.1 protein bound to hemocytes in vitro and in vivo and was endocytosed in a manner similar to the native protein produced in CsPDV-infected larvae. (C) 1997 Elsevier Science Ltd.

引用

页码：201 / 211

页数：11

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