Generation of RCAS vectors useful for functional genomic analyses.

S. Loftus, D. Larson, D. Watkins-Chow, D. Church, W. Pavan
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引用次数: 60

Abstract

Avian leukosis type A virus-derived retroviral vectors have been used to introduce genes into cells expressing the corresponding avian receptor tv-a. This includes the use of Replication-Competent Avian sarcoma-leukosis virus (ASLV) long terminal repeat (LTR) with Splice acceptor (RCAS) vectors in the analysis of avian development, human and murine cell cultures, murine cell lineage studies and cancer biology. Previously, cloning of genes into this virus was difficult due to the large size of the vector and sparse cloning sites. To overcome some of the disadvantages of traditional cloning using the RCASBP-Y vector, we have modified the RCASBP-Y to incorporate "Gateway" site-specific recombination cloning of genes into the construct, either with or without HA epitope tags. We have found the repetitive "att" sequences, which are the targets for site-specific recombination, do not impair the production of infectious viral particles or the expression of the gene of interest. This is the first instance of site-specific recombination being used to generate retroviral gene constructs. These viral constructs will allow for the efficient transfer and expression of cDNAs needed for functional genomic analyses.
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用于功能基因组分析的RCAS载体的生成。
禽白血病A型病毒衍生的逆转录病毒载体已被用于将基因导入表达相应禽受体tv-a的细胞中。这包括在鸟类发育、人类和小鼠细胞培养、小鼠细胞谱系研究和癌症生物学分析中使用复制能力禽流感肉瘤-白血病病毒(ASLV)长末端重复(LTR)与剪接受体(RCAS)载体。以前,由于载体体积大,克隆位点稀疏,将基因克隆到这种病毒中是困难的。为了克服使用RCASBP-Y载体进行传统克隆的一些缺点,我们对RCASBP-Y进行了修改,将“Gateway”位点特异性基因重组克隆加入到构建物中,无论是带HA表位标签还是不带HA表位标签。我们发现重复的“att”序列是位点特异性重组的目标,不会损害感染性病毒颗粒的产生或感兴趣基因的表达。这是第一次使用位点特异性重组来产生逆转录病毒基因结构。这些病毒结构将允许功能基因组分析所需的cdna的有效转移和表达。
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