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机构地区:[1]贵州省人民医院肝胆外科,贵州省贵阳市550002 [2]中国人民解放军第三军医大学西南医院全军肝胆外科,重庆市400038
出 处:《世界华人消化杂志》2008年第21期2337-2342,共6页World Chinese Journal of Digestology
基 金:贵州省优秀科技教育人才省长基金资助项目;No.2005-229~~
摘 要:目的:研究线粒体DNA上游调节基因mtTFA和NRF-1对冷保存肝移植大鼠肝细胞线粒体DNA ATPase6基因表达的影响,探讨mtTFA和NRF-1对冷保存肝移植大鼠肝细胞线粒体DNA调节作用及其机制.方法:Wistar大鼠186只,采用改良"二袖套法"制作大鼠肝移植模型,动物随机分为A组:冷保存30min;B组:冷保存6h;C组:冷保存12h;和D组(假手术对照组),分别于制模后于12h、24h、3d、5d、7d采集标本,保证每时相点存活大鼠6只.观察各组大鼠肝脏ATP含量.采用RT-PCR方法检测mtDNA ATPase6 mRNA、mtTFA和NRF-1 mRNA的表达变化.结果:冷保存再灌注后早期(12h),A、B、C三组mtTFA mRNA表达降低,与A、B组相比,C组最为显著(0.57±0.05vs0.87±0.11,0.69±0.10,P<0.05),NRF-1 mRNA表达变化与mtTFA mRNA相一致.24h后各组mtTFA及NRF-1 mRNA表达开始升高,ATPase6表达和肝组织ATP含量也升高,并且升高趋势与mtTFA及NRF-1 mRNA表达增高基本一致.结论:mtTFA和NRF-1可能通过基因转录调节ATPase6基因表达,改变线粒体呼吸链转运电子、合成ATP的能力.AIM: To observe the effects of mitochondrial transcription factor A (mtTFA) and nuclear respiratory factor-1 (NRF-1) on the expression of mitochondrial ATP6 genes during cold preservation and reperfusion injury in rats receiving orthotopic liver transplantation. METHODS: Orthotopic liver transplantation was performed in Wistar rats using the cuff technique as described by Kamada with modifications. A total of 186 rats were randomly divided into 4 groups, named as group A (30 min of cold preservation), group B (6 h of cold preservation), group C (12 h of cold preservation) and group D (sham operation). Hepatic samples were collected at 12 h, 24 h and on the 3^rd, 5^th, 7^th day after operation. The ATP levels were observed in each group. The expression levels of NRF-1, mtTFA and mtDNA encoding ATPase6 mRNA were determined by reverse transcription-polymerase chain reaction (RT-PCR). RESULTS: The expression of mtTFA decreased in groups A, B and C 12 h after operation, and it was lower in group C and groups A and B (0.57 ± 0.05 vs 0.87 ± 0.11, 0.69 ± 0.10, P 〈 0.05). The expression change of NRF-1 mRNA was consistent with that of mtTFA. After 24 h, the expression levels of mtTFA and NRF-1 mRNA started to increase, and the expression of ATPase6 mRNA and ATP in hepatic tissues were in accordance with mtTFA and NRF-1 mRNA. CONCLUSION: mtTFA and NRF-1 increase the expression of ATPase6 mRNA, suggesting mtTFA and NRF-1 may be important factors in controling ATPase6 mRNA transcription.
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