Enhanced design of pCMViR-TSC plasmid vector for sustainably high cargo gene expression in mammalian cells.

IF 1.5 4区生物学 Q4 CELL BIOLOGY

In Vitro Cellular & Developmental Biology. Animal Pub Date : 2024-12-01 Epub Date: 2024-11-21 DOI:10.1007/s11626-024-00992-2

Masakiyo Sakaguchi, Rie Kinoshita, Nahoko Tomonobu, Yoshihiko Sakaguchi, Junichiro Futami, Akira Yamauchi, Hitoshi Murata, Ken-Ichi Yamamoto, Tetta Takahashi, Yuma Gohara, Toshiki Ochi, Fan Jiang, Ni Luh Gede Yoni Komalasari, Youyi Chen, I Made Winarsa Ruma, I Wayan Sumardika, Jin Zhou, Tomoko Honjo, Futoshi Kuribayashi, Kazumi Sagayama, Shinichi Toyooka, Eisaku Kondo, Yusuke Inoue

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引用次数: 0

Abstract

The first-generation pCMViR-TSC, implemented through the promoter sandwich rule, yields 10- to 100-fold higher gene expression than the standard plasmid used with the CMV (cytomegalovirus) or CAG promoter. However, the vector's shortcomings limit its utility to transient expression only, as it is not suitable for establishing stable transformants in mammalian cells. To overcome this weakness, we here introduce the improved plasmid vector pSAKA-4B, derived from pCMViR-TSC as a second-generation chromosome-insertable vector. This vector facilitates the linear entry of the expression unit into the TTAA site of DNA universally with transposase assistance. The vector is helpful for the indefinite expression of our target gene. The new vector system is proven here to be efficient in establishing stable transformants with a high likelihood of positive clones that exhibit significantly elevated expression levels of the delivered foreign gene. This system, alongside the first-generation vector, is therefore instrumental for diverse basic research endeavors concerning genes, proteins, cells, and animals, and potentially for clinical applications such as gene therapy.

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改进 pCMViR-TSC 质粒载体的设计，实现哺乳动物细胞中可持续的高负载基因表达。

与使用 CMV（巨细胞病毒）或 CAG 启动子的标准质粒相比，通过启动子三明治规则实现的第一代 pCMViR-TSC 基因表达量高出 10 到 100 倍。然而，该载体的缺点限制了它只能用于瞬时表达，因为它不适合在哺乳动物细胞中建立稳定的转化体。为了克服这一缺陷，我们在此引入了改进的质粒载体 pSAKA-4B，它源自 pCMViR-TSC，是第二代染色体可插入载体。在转座酶的帮助下，该载体能使表达单元线性地进入 DNA 的 TTAA 位点。该载体有助于目标基因的无限表达。事实证明，新的载体系统能有效地建立稳定的转化体，并极有可能产生阳性克隆，从而显著提高外来基因的表达水平。因此，该系统与第一代载体一起，有助于开展有关基因、蛋白质、细胞和动物的各种基础研究工作，并有可能用于基因治疗等临床应用。

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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来源期刊

In Vitro Cellular & Developmental Biology. Animal 生物-发育生物学

CiteScore

3.70

自引率

4.80%

发文量

审稿时长

3 months

期刊介绍： In Vitro Cellular & Developmental Biology - Animal is a journal of the Society for In Vitro Biology (SIVB). Original manuscripts reporting results of research in cellular, molecular, and developmental biology that employ or are relevant to organs, tissue, tumors, and cells in vitro will be considered for publication. Topics covered include: Biotechnology; Cell and Tissue Models; Cell Growth/Differentiation/Apoptosis; Cellular Pathology/Virology; Cytokines/Growth Factors/Adhesion Factors; Establishment of Cell Lines; Signal Transduction; Stem Cells; Toxicology/Chemical Carcinogenesis; Product Applications.