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启动子优化绕过 Bcl-2 转基因介导的慢病毒载体生产抑制。

Promoter Optimization Circumvents Bcl-2 Transgene-Mediated Suppression of Lentiviral Vector Production.

机构信息

Centre for Heart Research, The Westmead Institute for Medical Research, Westmead, NSW 2145, Australia.

Westmead Clinical School, The University of Sydney, Westmead, NSW 2145, Australia.

出版信息

Biomolecules. 2023 Sep 16;13(9):1397. doi: 10.3390/biom13091397.

Abstract

Lentiviral vectors are a robust gene delivery tool for inducing transgene expression in a variety of cells. They are well suited to facilitate the testing of therapeutic candidate genes in vitro, due to relative ease of packaging and ability to transduce dividing and non-dividing cells. Our goal was to identify a gene that could be delivered to the heart to protect against cancer-therapy-induced cardiotoxicity. We sought to generate a lentivirus construct with a ubiquitous CMV promoter driving expression of B-cell lymphocyte/leukemia 2 gene (), a potent anti-apoptotic gene. Contrary to our aim, overexpression of Bcl-2 induced cell death in the producer HEK293T cells, resulting in failure to produce usable vector titre. This was circumvented by exchanging the CMV promoter to the cardiac-specific NCX1 promoter, leading to the successful production of a lentiviral vector which could induce cardioprotective expression of Bcl-2. In conclusion, reduced expression of Bcl-2 driven by a weaker promoter improved vector yield, and led to the production of functional cardioprotective Bcl-2 in primary cardiomyocytes.

摘要

慢病毒载体是一种强大的基因传递工具,可在多种细胞中诱导转基因表达。由于相对容易包装和能够转导分裂和非分裂细胞,因此非常适合在体外测试治疗候选基因。我们的目标是鉴定一种可递送到心脏以预防癌症治疗引起的心脏毒性的基因。我们试图生成一种带有普遍 CMV 启动子的慢病毒构建体,驱动 B 细胞淋巴细胞/白血病 2 基因 () 的表达,这是一种有效的抗凋亡基因。与我们的目标相反,Bcl-2 的过表达导致产生细胞死亡的生产者 HEK293T 细胞,导致无法生产可用的载体效价。通过将 CMV 启动子交换为心脏特异性 NCX1 启动子来规避这一问题,从而成功生产出能够诱导 Bcl-2 心脏保护表达的慢病毒载体。总之,由较弱的启动子驱动的 Bcl-2 表达减少提高了载体产量,并导致在原代心肌细胞中产生功能性的心脏保护 Bcl-2。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/b454/10526134/6edccc875716/biomolecules-13-01397-g001.jpg

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