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优化基于质粒的基因转移以研究骨骼肌结构和功能。

Optimizing plasmid-based gene transfer for investigating skeletal muscle structure and function.

作者信息

Schertzer Jonathan D, Plant David R, Lynch Gordon S

机构信息

Department of Physiology, The University of Melbourne, Melbourne, VIC 3010, Australia.

出版信息

Mol Ther. 2006 Apr;13(4):795-803. doi: 10.1016/j.ymthe.2005.09.019. Epub 2005 Nov 23.

DOI:10.1016/j.ymthe.2005.09.019
PMID:16309967
Abstract

Intramuscular injection of naked plasmid DNA is a less cytotoxic alternative to viral vectors for delivering genetic material to skeletal muscle in vivo. However, the low efficiency of plasmid-based gene transfer limits its potential therapeutic efficacy and/or its use for many experimental applications. Current strategies to enhance transfection efficiency (i.e., electroporation) can cause significant muscle damage, confounding physiological assessments such as muscle contractility. Optimizing protocols to limit damage is critical for accurate physiological, biochemical, and molecular measurements. Following extensive testing, we developed an electroporation protocol that enhances transfection efficiency in skeletal muscles without causing muscle damage. Pretreating mouse tibialis anterior muscles with hyaluronidase and electroporation at 75 V/cm (using 50% vol/vol saline as a vehicle for plasmid DNA) resulted in 22 +/- 5% of the muscle fibers expressing a reporter gene. This protocol did not compromise contractile function of skeletal muscles assessed at both the intact (whole) muscle and the cellular (single fiber) level. Furthermore, ectopic expression of insulin-like growth factor I to levels that induced muscle fiber hypertrophy without causing tissue damage or compromising muscle function highlights the therapeutic potential of these methods for myopathies, muscle wasting disorders, and other pathophysiologic conditions.

摘要

肌肉内注射裸质粒DNA是一种在体内将遗传物质传递到骨骼肌的细胞毒性低于病毒载体的替代方法。然而,基于质粒的基因转移效率低下限制了其潜在的治疗效果和/或在许多实验应用中的使用。当前提高转染效率的策略(如电穿孔)会导致明显的肌肉损伤,干扰诸如肌肉收缩性等生理评估。优化方案以限制损伤对于准确的生理、生化和分子测量至关重要。经过广泛测试,我们开发了一种电穿孔方案,可提高骨骼肌的转染效率而不引起肌肉损伤。用透明质酸酶预处理小鼠胫前肌并在75 V/cm下进行电穿孔(使用50%体积/体积的盐水作为质粒DNA的载体),导致22±5%的肌纤维表达报告基因。该方案在完整(整体)肌肉和细胞(单纤维)水平评估时均未损害骨骼肌的收缩功能。此外,胰岛素样生长因子I异位表达至诱导肌纤维肥大的水平,且未引起组织损伤或损害肌肉功能,这突出了这些方法对肌病、肌肉萎缩症及其他病理生理状况的治疗潜力。

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Hyaluronidase impacts exposures of long-acting injectable paliperidone palmitate in rodent models.透明质酸酶影响长效注射用棕榈酸帕利哌酮在啮齿动物模型中的暴露量。
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