Hojman Pernille, Zibert John R, Gissel Hanne, Eriksen Jens, Gehl Julie
Laboratory of the Department of Oncology, Copenhagen University Hospital Herlev, Herlev, Denmark.
BMC Mol Biol. 2007 Jun 29;8:56. doi: 10.1186/1471-2199-8-56.
Gene transfer by electroporation (DNA electrotransfer) to muscle results in high level long term transgenic expression, showing great promise for treatment of e.g. protein deficiency syndromes. However little is known about the effects of DNA electrotransfer on muscle fibres. We have therefore investigated transcriptional changes through gene expression profile analyses, morphological changes by histological analysis, and physiological changes by force generation measurements. DNA electrotransfer was obtained using a combination of a short high voltage pulse (HV, 1000 V/cm, 100 mus) followed by a long low voltage pulse (LV, 100 V/cm, 400 ms); a pulse combination optimised for efficient and safe gene transfer. Muscles were transfected with green fluorescent protein (GFP) and excised at 4 hours, 48 hours or 3 weeks after treatment.
Differentially expressed genes were investigated by microarray analysis, and descriptive statistics were performed to evaluate the effects of 1) electroporation, 2) DNA injection, and 3) time after treatment. The biological significance of the results was assessed by gene annotation and supervised cluster analysis.Generally, electroporation caused down-regulation of structural proteins e.g. sarcospan and catalytic enzymes. Injection of DNA induced down-regulation of intracellular transport proteins e.g. sentrin. The effects on muscle fibres were transient as the expression profiles 3 weeks after treatment were closely related with the control muscles. Most interestingly, no changes in the expression of proteins involved in inflammatory responses or muscle regeneration was detected, indicating limited muscle damage and regeneration. Histological analysis revealed structural changes with loss of cell integrity and striation pattern in some fibres after DNA+HV+LV treatment, while HV+LV pulses alone showed preservation of cell integrity. No difference in the force generation capacity was observed in the muscles 2 weeks after DNA electrotransfer.
The small and transient changes found in the gene expression profiles are of great importance, as this demonstrates that DNA electrotransfer is safe with minor effects on the muscle host cells. These findings are essential for introducing the DNA electrotransfer to muscle for clinical use. Indeed the HV+LV pulse combination used has been optimised to ensure highly efficient and safe DNA electrotransfer.
通过电穿孔法(DNA 电转染)将基因导入肌肉可实现高水平的长期转基因表达,这在治疗例如蛋白质缺乏综合征等方面展现出巨大潜力。然而,关于 DNA 电转染对肌纤维的影响却知之甚少。因此,我们通过基因表达谱分析研究转录变化,通过组织学分析研究形态变化,并通过力量产生测量研究生理变化。使用短高压脉冲(HV,1000 V/cm,100 μs)随后接长低压脉冲(LV,100 V/cm,400 ms)的组合来实现 DNA 电转染;这种脉冲组合是为高效且安全的基因转移而优化的。用绿色荧光蛋白(GFP)转染肌肉,并在处理后 4 小时、48 小时或 3 周切除。
通过微阵列分析研究差异表达基因,并进行描述性统计以评估 1)电穿孔、2)DNA 注射和 3)处理后时间的影响。通过基因注释和监督聚类分析评估结果的生物学意义。一般来说,电穿孔导致结构蛋白如肌膜相关蛋白和催化酶的下调。注射 DNA 诱导细胞内转运蛋白如泛素缀合酶的下调。对肌纤维的影响是短暂的,因为处理后 3 周的表达谱与对照肌肉密切相关。最有趣的是,未检测到参与炎症反应或肌肉再生的蛋白质表达有变化,表明肌肉损伤和再生有限。组织学分析显示,在 DNA + HV + LV 处理后,一些纤维出现细胞完整性丧失和条纹模式改变的结构变化,而单独的 HV + LV 脉冲显示细胞完整性得以保留。DNA 电转染后 2 周,肌肉的力量产生能力未观察到差异。
在基因表达谱中发现的微小且短暂的变化非常重要,因为这表明 DNA 电转染是安全的,对肌肉宿主细胞影响较小。这些发现对于将 DNA 电转染引入肌肉用于临床应用至关重要。实际上,所使用的 HV + LV 脉冲组合已进行优化,以确保高效且安全的 DNA 电转染。
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