插入序列长度决定了双链哺乳动物表达载体的转染效率和基因表达水平。

International journal of biochemistry and molecular biology Pub Date : 2013-12-15 eCollection Date: 2013-01-01
Andrew J Payne, Bryan C Gerdes, Simon Kaja, Peter Koulen
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引用次数: 0

摘要

自25年前首次发现内部核糖体进入位点(IRES)以来,双链表达载体已被广泛用于共表达研究。IRES序列允许在单个信使RNA链上的多个基因的5'帽独立的翻译起始。利用市购的含有3'绿色荧光蛋白荧光标记的IRES序列的哺乳动物表达载体,我们发现IRES位点上表达的目标基因的5'序列长度影响3'荧光标记的表达和载体构建的整体转染效率。此外,我们产生了一种表达两种不同荧光标记的新结构,并发现一个基因的高表达可以降低另一个基因的表达。本研究的观察结果表明,在使用具有短5'基因序列的IRES系统进行实验设计时需要谨慎(
本文章由计算机程序翻译,如有差异,请以英文原文为准。

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Insert sequence length determines transfection efficiency and gene expression levels in bicistronic mammalian expression vectors.

Bicistronic expression vectors have been widely used for co-expression studies since the initial discovery of the internal ribosome entry site (IRES) about 25 years ago. IRES sequences allow the 5' cap-independent initiation of translation of multiple genes on a single messenger RNA strand. Using a commercially available mammalian expression vector containing an IRES sequence with a 3' green fluorescent protein fluorescent marker, we found that sequence length of the gene of interest expressed 5' of the IRES site influences both expression of the 3' fluorescent marker and overall transfection efficiency of the vector construct. Furthermore, we generated a novel construct expressing two distinct fluorescent markers and found that high expression of one gene can lower expression of the other. Observations from this study indicate that caution is warranted in the design of experiments utilizing an IRES system with a short 5' gene of interest sequence (<300 bp), selection of single cells based on the expression profile of the 3' optogenetic fluorescent marker, and assumptions made during data analysis.

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