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构建杆状病毒-家蚕多基因表达系统及其在生产病毒样颗粒中的应用。

Construction of a baculovirus-silkworm multigene expression system and its application on producing virus-like particles.

机构信息

China-United Kingdom Nanyang Normal University-Rothamsted Research Joint Laboratory of Insect Biology, Henan Provincial Key Laboratory of Funiu Mountain Insect Biology, Nanyang Normal University, Nanyang, People's Republic of China.

出版信息

PLoS One. 2012;7(3):e32510. doi: 10.1371/journal.pone.0032510. Epub 2012 Mar 5.

Abstract

A new baculovirus-silkworm multigene expression system named Bombyx mori MultiBac is developed and described here, by which multiple expression cassettes can be introduced into the Bombyx mori nuclear polyhedrosis virus (BmNPV) genome efficiently. The system consists of three donor vectors (pCTdual, pRADM and pUCDMIG) and an invasive diaminopimelate (DAP) auxotrophic recipient E. coli containing BmNPV-Bacmid (BmBacmid) with a homologous recombination region, an attTn7 site and a loxp site. Two genes carried by pCTdual are firstly inserted into BmBacmid by homologous recombination, while the other eight genes in pRADM and pUCDMIG are introduced into BmBacmid through Tn7 transposition and cre-loxp recombination. Then the invasive and DAP auxotrophic E. coli carrying recombinant BmBacmid is directly injected into silkworm for expressing heterologous genes in larvae or pupae. Three structural genes of rotavirus and three fluorescent genes have been simultaneously expressed in silkworm larvae using our new system, resulting in the formation of virus-like particles (VLPs) of rotavirus and the color change of larvae. The VLPs were purified from hemolymph by ultracentrifugation using CsCl gradients, with a yield of 12.7 µg per larva. For the great capacity of foreign genes and the low cost of feeding silkworm, this high efficient BmMultiBac expression system provides a suitable platform to produce VLPs or protein complexes.

摘要

我们开发并描述了一种新的杆状病毒-家蚕多基因表达系统,命名为 Bombyx mori MultiBac,它可以有效地将多个表达盒引入家蚕核型多角体病毒(BmNPV)基因组中。该系统由三个供体载体(pCTdual、pRADM 和 pUCDMIG)和一个含有 BmNPV-Bacmid(BmBacmid)的入侵二氨基庚二酸(DAP)营养缺陷型受体大肠杆菌组成,BmBacmid 带有同源重组区、attTn7 位点和 loxp 位点。pCTdual 携带的两个基因首先通过同源重组插入 BmBacmid,而 pRADM 和 pUCDMIG 中的另外八个基因则通过 Tn7 转座和 cre-loxp 重组插入 BmBacmid。然后将携带重组 BmBacmid 的入侵和 DAP 营养缺陷型大肠杆菌直接注射到家蚕体内,在幼虫或蛹中表达异源基因。使用我们的新系统,三种轮状病毒结构基因和三种荧光基因在家蚕幼虫中同时表达,导致轮状病毒样颗粒(VLPs)的形成和幼虫颜色的变化。VLPs 可以通过 CsCl 梯度超速离心从血液中纯化出来,每条幼虫的产量为 12.7 µg。由于该系统具有大容量的外源基因和低成本的饲养家蚕的优势,因此这种高效的 BmMultiBac 表达系统为生产 VLPs 或蛋白质复合物提供了一个合适的平台。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e6fd/3293821/2fcb16a1db30/pone.0032510.g001.jpg

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