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从携带完整人类基因和相关调控元件的 BAC 载体中表达 CFTR。

CFTR expression from a BAC carrying the complete human gene and associated regulatory elements.

机构信息

Department of Histology and Embryology, School of Medicine, University of Athens, Athens, Greece.

出版信息

J Cell Mol Med. 2009 Sep;13(9A):2938-48. doi: 10.1111/j.1582-4934.2008.00433.x. Epub 2008 Jul 24.

Abstract

The use of genomic DNA rather than cDNA or mini-gene constructs in gene therapy might be advantageous as these contain intronic and long-range control elements vital for accurate expression. For gene therapy of cystic fibrosis though, no bacterial artificial chromosome (BAC), containing the whole CFTR gene is available. We have used Red homologous recombination to add a to a previously described vector to construct a new BAC vector with a 250.3-kb insert containing the whole coding region of the CFTR gene along with 40.1 kb of DNA 5' to the gene and 25 kb 3' to the gene. This includes all the known control elements of the gene. We evaluated expression by RT-PCR in CMT-93 cells and showed that the gene is expressed both from integrated copies of the BAC and also from episomes carrying the oriP/EBNA-1 element. Sequencing of the human CFTR mRNA from one clone showed that the BAC is functional and can generate correctly spliced mRNA in the mouse background. The BAC described here is the only CFTR genomic construct available on a convenient vector that can be readily used for gene expression studies or in vivo studies to test its potential application in gene therapy for cystic fibrosis.

摘要

使用基因组 DNA 而不是 cDNA 或微基因构建体进行基因治疗可能是有利的,因为这些构建体包含对于准确表达至关重要的内含子和长距离调控元件。 然而,对于囊性纤维化的基因治疗,没有包含整个 CFTR 基因的细菌人工染色体(BAC)可用。 我们使用 Red 同源重组技术在先前描述的载体上添加一个,构建了一个新的 BAC 载体,该载体包含全长 CFTR 基因的 250.3-kb 插入片段,以及基因 5'端的 40.1 kb DNA 和基因 3'端的 25 kb。 这包括该基因的所有已知调控元件。 我们通过 RT-PCR 在 CMT-93 细胞中评估了表达情况,并表明该基因既可以从 BAC 的整合拷贝中表达,也可以从携带 oriP/EBNA-1 元件的附加体中表达。 对一个克隆的人类 CFTR mRNA 进行测序表明,BAC 是功能性的,可以在小鼠背景下产生正确剪接的 mRNA。 本文描述的 BAC 是唯一可在方便的载体上获得的 CFTR 基因组构建体,可用于基因表达研究或体内研究,以测试其在囊性纤维化基因治疗中的潜在应用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1f47/4498948/66e167f84695/jcmm0013-2938-f1.jpg

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