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重组逆转录病毒的产生及对B细胞的感染。

Recombinant retroviral production and infection of B cells.

作者信息

Keim Celia, Grinstein Veronika, Basu Uttiya

机构信息

Department of Microbiology and Immunology, Columbia University College of Physicians and Surgeons, USA.

出版信息

J Vis Exp. 2011 Feb 18(48):2371. doi: 10.3791/2371.

Abstract

The transgenic expression of genes in eukaryotic cells is a powerful reverse genetic approach in which a gene of interest is expressed under the control of a heterologous expression system to facilitate the analysis of the resulting phenotype. This approach can be used to express a gene that is not normally found in the organism, to express a mutant form of a gene product, or to over-express a dominant-negative form of the gene product. It is particularly useful in the study of the hematopoietic system, where transcriptional regulation is a major control mechanism in the development and differentiation of B cells, reviewed. Mouse genetics is a powerful tool for the study of human genes and diseases. A comparative analysis of the mouse and human genome reveals conservation of synteny in over 90% of the genome. Also, much of the technology used in mouse models is applicable to the study of human genes, for example, gene disruptions and allelic replacement. However, the creation of a transgenic mouse requires a great deal of resources of both a financial and technical nature. Several projects have begun to compile libraries of knock out mouse strains (KOMP, EUCOMM, NorCOMM) or mutagenesis induced strains (RIKEN), which require large-scale efforts and collaboration. Therefore, it is desirable to first study the phenotype of a desired gene in a cell culture model of primary cells before progressing to a mouse model. Retroviral DNA integrates into the host DNA, preferably within or near transcription units or CpG islands, resulting in stable and heritable expression of the packaged gene of interest while avoiding transcriptional silencing. The genes are then transcribed under the control of a high efficiency retroviral promoter, resulting in a high efficiency of transcription and protein production. Therefore, retroviral expression can be used with cells that are difficult to transfect, provided the cells are in an active state during mitosis. Because the structural genes of the virus are contained within the packaging cell line, the expression vectors used to clone the gene of interest contain no structural genes of the virus, which both eliminates the possibility of viral revertants and increases the safety of working with viral supernatants as no infectious virions are produced. Here we present a protocol for recombinant retroviral production and subsequent infection of splenic B cells. After isolation, the cultured splenic cells are stimulated with Th derived lymphokines and anti-CD40, which induces a burst of B cell proliferation and differentiation. This protocol is ideal for the study of events occurring late in B cell development and differentiation, as B cells are isolated from the spleen following initial hematopoietic events but prior to antigenic stimulation to induce plasmacytic differentiation.

摘要

真核细胞中基因的转基因表达是一种强大的反向遗传学方法,其中目的基因在异源表达系统的控制下表达,以促进对所得表型的分析。这种方法可用于表达生物体中通常不存在的基因、表达基因产物的突变形式或过表达基因产物的显性负性形式。它在造血系统研究中特别有用,在造血系统中,转录调控是B细胞发育和分化的主要控制机制(已综述)。小鼠遗传学是研究人类基因和疾病的有力工具。对小鼠和人类基因组的比较分析表明,超过90%的基因组存在同线性保守性。此外,小鼠模型中使用的许多技术也适用于人类基因研究,例如基因敲除和等位基因替换。然而,创建转基因小鼠需要大量的资金和技术资源。几个项目已经开始编制基因敲除小鼠品系文库(KOMP、EUCOMM、NorCOMM)或诱变诱导品系文库(理化学研究所),这需要大规模的努力和合作。因此,在进入小鼠模型之前,最好先在原代细胞的细胞培养模型中研究目的基因的表型。逆转录病毒DNA整合到宿主DNA中,最好是在转录单元或CpG岛内部或附近,从而导致包装的目的基因稳定且可遗传地表达,同时避免转录沉默。然后,基因在高效逆转录病毒启动子的控制下转录,从而实现高效转录和蛋白质产生。因此,只要细胞在有丝分裂期间处于活跃状态,逆转录病毒表达就可用于难以转染的细胞。由于病毒的结构基因包含在包装细胞系中,用于克隆目的基因的表达载体不包含病毒的结构基因,这既消除了病毒回复突变体的可能性,又提高了使用病毒上清液的安全性,因为不会产生感染性病毒粒子。在此,我们介绍一种重组逆转录病毒生产及随后感染脾B细胞的方案。分离后,用Th衍生的淋巴因子和抗CD40刺激培养的脾细胞,这会诱导B细胞增殖和分化爆发。该方案非常适合研究B细胞发育和分化后期发生的事件,因为B细胞是在初始造血事件之后但在抗原刺激诱导浆细胞分化之前从脾脏中分离出来的。

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