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与生物素诱饵共表达 BirA 可实现转基因家蚕中超表达稳定 N-糖基化 sRAGE 的体内生物素化。

Co-expression of BirA with biotin bait achieves in vivo biotinylation of overexpressed stable N-glycosylated sRAGE in transgenic silkworms.

机构信息

Food Research Institute, NARO, 2-1-12 Kannondai, Tsukuba, Ibaraki, 305-8642, Japan.

Institute of Agrobiological Sciences, NARO, 1-2 Owashi, Tsukuba, Ibaraki, 305-8643, Japan.

出版信息

Sci Rep. 2017 Mar 23;7(1):356. doi: 10.1038/s41598-017-00420-4.

Abstract

Here, we demonstrated the expression of the N-glycosylated extracellular ligand binding domain of receptor for advanced glycation end products (sRAGE) in middle silk glands (MSGs) of transgenic silkworms using the GAL4/UAS system. Over 1 mg of sRAGE was obtained from one transgenic silkworm. sRAGE purified from the silkworm exhibited good stability and maintained specific ligand-binding ability. In addition, N-glycan analysis of sRAGE revealed that N-glucan completely lacked potentially allergenic fucose. Moreover, co-expression of biotin ligase (BirA) with C-terminal BioEase-tagged sRAGE in MSGs resulted in efficient biotinylation of sRAGE after addition of biotin bait. C-terminal biotinylated sRAGE could be immobilized onto a solid surface in one direction through binding to streptavidin without any loss of ability. The dissociation constant of sRAGE with fructose-BSA, a typical RAGE ligand, was 7.25 × 10 M, consistent with that on the mammalian cell surface. Thus, we developed a novel, innovative silkworm expression system for efficient expression of recombinant sRAGE, which could serve as a basis for the elucidation of RAGE-ligand interactions and facilitate the search for new ligands and inhibitors.

摘要

在这里,我们使用 GAL4/UAS 系统展示了在转基因家蚕的中丝腺(MSGs)中表达糖基化末端产物受体的 N-糖基化细胞外配体结合域(sRAGE)。从一只转基因家蚕中获得了超过 1mg 的 sRAGE。从家蚕中纯化出的 sRAGE 表现出良好的稳定性,并保持了特定的配体结合能力。此外,sRAGE 的 N-聚糖分析表明,N-葡聚糖完全缺乏潜在的过敏原岩藻糖。此外,在 MSGs 中与 C 末端 BioEase 标记的 sRAGE 共表达生物素连接酶(BirA)后,添加生物素诱饵可使 sRAGE 有效生物素化。C 末端生物素化的 sRAGE 可以通过与链霉亲和素结合而在一个方向上固定在固体表面上,而不会丧失任何能力。sRAGE 与果糖-BSA(一种典型的 RAGE 配体)的解离常数为 7.25×10^-7M,与哺乳动物细胞表面上的解离常数一致。因此,我们开发了一种新型的、创新的家蚕表达系统,用于高效表达重组 sRAGE,这可以为阐明 RAGE-配体相互作用提供基础,并有助于寻找新的配体和抑制剂。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/40fb/5428419/0f202ceb00dc/41598_2017_420_Fig1_HTML.jpg

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