Transgenic mice Cre-dependently expressing mutant polymerase-gamma: novel test-system for pharmacological study of mitoprotective drugs

Q3 Pharmacology, Toxicology and Pharmaceutics
M. Kubekina, Y. Silaeva, A. Bruter, D. Korshunova, L. Ilchuk, Yulia D. Okulova, M. O. Soldatova, E. Seryogina, I. Kolesnik, Polina A. Ukolova, M. Korokin, A. Deykin
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引用次数: 4

Abstract

Introduction: PolG-alpha is a nuclear-encoded enzyme which provides replication and repair of mitochondrial DNA. D257A mutation of PolG-alpha leads to change in the N-terminal ”proofreading” domain, which deprives the enzyme of 3′-5′ exonuclease activity, resulting in accumulation of mutations in the mitochondrial genome. Materials and methods: Murine zygotes were microinjected with transgene construction carrying mutant murine Polg coding sequence and GFP coding sequence by a loxP-flanked STOP-cassette. Two Cre-activator strains, CMV-Cre (systemic activation) and Tie2-Cre (endothelial activation), were used for activation of the transgene. To confirm the insertion and Cre-dependent activation of the transgene, genotyping and qPCR copy number measurement of mutant Polg were performed, and GFP fluorescence was assessed. Results: Two primary transgenic animals were used as the founders for two lines with copy numbers of transgene ~7 and ~5. After systemic activation, the number of the transgene copies decreases to ~1.0 while endothelial specific activation does not affect the number of transgene copies in tail tissue. Discussion: A murine model with spatial control of mutant Polg expression has been developed. To our knowledge, this is the first transgenic model of tissue-specific mitochondrial dysfunction. Conclusion: Transgenic mice Cre-dependent expressing mutant polymerase-gamma are a novel test-system for studying mitochondrial biology and efficacy of mitoprotective drugs.
表达突变型聚合酶γ的转基因小鼠:线粒体保护药物药理研究的新测试系统
引言:PolG-alpha是一种核编码酶,可提供线粒体DNA的复制和修复。PolGα的D257A突变导致N端“校对”结构域的变化,从而剥夺了该酶的3′-5′核酸外切酶活性,导致线粒体基因组中突变的积累。材料和方法:通过loxP侧翼的STOP盒,用携带突变小鼠Polg编码序列和GFP编码序列的转基因构建物微注射小鼠受精卵。两种Cre激活剂菌株,CMV-Cre(全身激活)和Tie2-Cre(内皮激活),用于转基因的激活。为了确认转基因的插入和Cre依赖性激活,对突变体Polg进行基因分型和qPCR拷贝数测量,并评估GFP荧光。结果:用两个原代转基因动物作为两个品系的建立者,转基因拷贝数分别为~7和~5。全身激活后,转基因拷贝数降至约1.0,而内皮特异性激活不影响尾部组织中转基因拷贝数。讨论:已经建立了一种具有突变体Polg表达空间控制的小鼠模型。据我们所知,这是第一个组织特异性线粒体功能障碍的转基因模型。结论:表达Cre依赖性突变聚合酶γ的转基因小鼠是研究线粒体生物学和线粒体保护药物疗效的一种新的检测系统。
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
Research Results in Pharmacology
Research Results in Pharmacology Medicine-Pharmacology (medical)
CiteScore
1.50
自引率
0.00%
发文量
32
审稿时长
12 weeks
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