成年兔心肌肥厚性心肌病突变的体内短期表达:无早期紊乱的肌纤维掺入。

Q Yu, G Zhao, A J Marian
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引用次数: 7

摘要

心肌细胞紊乱是肥厚性心肌病(HCM)的病理标志,肥厚性心肌病是一种肉瘤蛋白疾病。心肌肌钙蛋白T (cTnT)是导致HCM的主要基因,其突变与严重的心肌细胞紊乱有关。为了研究心肌细胞紊乱的发病机制,我们通过在成年兔心肌内直接注射重组腺病毒来表达正常和突变的cTnT蛋白。将等量的1010个斑块形成单位的正常(Ad/CMV/cTnT-Arg92)和突变(Ad/CMV/cTnT-Gln92)重组病毒或对照载体(Ad/DeltaE)病毒与等量的报告病毒(Ad/CMV/Lac-Z)混合,共同注射到成年兔的心肌中(n = 12)。基因转移一周后,取心肌薄片,分析β -半乳糖苷酶、信使RNA (mRNA)和蛋白表达、苏木精和伊红、马松三色、免疫荧光染色和电镜。在长度约为2.5 mm的区域内,基因转移的效率从2%到60%不等。Northern blotting证实转基因表达为mRNA。肌原纤维蛋白提取物的免疫印迹和间接免疫荧光染色证实了转基因蛋白在肌原纤维中的表达和掺入。突变体cTnT的表达量高达内源性的18%。光镜和电镜检查显示心肌细胞和肌节结构正常。因此,尽管加入了突变体cTnT-Gln92,体内仍能进行稳定的肌原纤维形成和肌节组装。肌细胞和肌瘤紊乱的缺失可能反映了突变体cTnT-Gln92的持续时间、表达水平或肌纤维结合的程度,以及转基因表达的位置和时间,以及HCM发病机制中的种间变异。
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In vivo short-term expression of a hypertrophic cardiomyopathy mutation in adult rabbit myocardium: myofibrillar incorporation without early disarray.

Cardiac myocyte disarray is the pathological hallmark of hypertrophic cardiomyopathy (HCM), a disease of sarcomeric proteins. Mutations in the cardiac troponin T (cTnT), a major gene responsible for HCM, are associated with severe myocyte disarray. To study the pathogenesis of cardiac myocyte disarray, we expressed normal and mutant cTnT proteins in the myocardium of adult rabbits via direct intramyocardial injection of recombinant adenoviruses. Aliquots of 1010 plaque-forming units of normal (Ad/CMV/cTnT-Arg92) and mutant (Ad/CMV/cTnT-Gln92) recombinant viruses or a control vector (Ad/DeltaE) virus were mixed with equal aliquots of a reporter virus (Ad/CMV/Lac-Z) and co-injected into the myocardium of adult rabbits (n = 12). One week following gene transfer, thin myocardial sections were obtained and analyzed for beta-galactosidase, messenger RNA (mRNA) and protein expression, hematoxylin and eosin, Masson's trichrome, immunofluorescence staining, and electron microscopy. The efficiency of gene transfer varied from 2% to 60% of the cells in an area approximately 2.5 mm in length. Northern blotting confirmed expression of the transgenes into mRNA. Immunoblotting of the myofibrillar protein extracts and indirect immunofluorescence staining confirmed expression and incorporation of the transgene proteins into myofibrils. Expression of the mutant cTnT was up to 18% of the endogenous. Light and electron microscopic studies showed normal cardiac myocyte and sarcomere structures. Thus, despite incorporation of the mutant cTnT-Gln92, stable myofibrillar formation and sarcomere assembly proceeded in vivo. The absence of myocyte and sarcomere disarray may reflect the duration, or the level of expression, or the extent of myofibrillar incorporation of the mutant cTnT-Gln92, as well as the site and timing of expression of the transgenes, and interspecies variation in the pathogenesis of HCM.

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