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首页> 外文期刊>Journal of vascular surgery >Isolation of genes differentially expressed at the downstream anastomosis of prosthetic arterial grafts with use of mRNA differential display.
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Isolation of genes differentially expressed at the downstream anastomosis of prosthetic arterial grafts with use of mRNA differential display.

机译:利用mRNA差异显示技术分离假体动脉移植物下游吻合处差异表达的基因。

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摘要

PURPOSE: Downstream anastomotic intimal hyperplasia in prosthetic arterial grafts remains a major cause of delayed graft failure. The new method of messenger RNA (mRNA) differential display was used to screen numerous genes to gain insight into the molecular mechanisms of intimal hyperplasia. METHODS: Fifty-centimeter-long 8 mm expanded polytetrafluoroethylene grafts were placed in four mongrel dogs from the carotid artery to the distal abdominal aorta. At 3 months the distal anastomoses and adjacent normal aortas were harvested; a portion was taken for histologic examination, and total RNA was isolated from the remainder. Differential mRNA display was used to identify candidate cDNA clones whose expression differed in anastomotic intimal hyperplasia as compared with adjacent unaffected aorta. The clones were sequenced, and national gene databases were searched. Northern blot analysis confirmed alteration of gene expression. RESULTS: Approximately 5000 mRNA species were screened, and 11 candidate clones were obtained. DNA sequence revealed homology of five clones to known gene sequences. Homologous genes included an interferon-gamma-induced human gene, (IGUP I-5111), alpha-1 protease inhibitor gene, human retinoblastoma susceptibility gene, and human creatine kinase gene (two clones). Northern blot analysis revealed altered gene expression in 4 of 11, nonregulation in 1 of 11, and undetectable signals in 6 of 11. Expression of the clone representing IGUP I-5111 in the segment of intimal hyperplasia was found to be decreased over threefold to only 31% +/- 16.4% SE of the level seen in normal aorta. CONCLUSIONS: The technique of mRNA differential display has identified differences in gene expression in an in vivo model of anastomotic intimal hyperplasia. Expression of RNA with homology to an interferon-gamma-induced human gene was consistently decreased within the hyperplastic region at the downstream polytetrafluoroethylene arterial anastomosis.
机译:目的:人工动脉移植物中的下游吻合内膜增生仍然是延迟移植失败的主要原因。信使RNA(mRNA)差异显示的新方法用于筛选众多基因,以深入了解内膜增生的分子机制。方法:将五十厘米长的8 mm扩展聚四氟乙烯移植物从颈动脉到腹主动脉远端放置在四只杂种狗中。 3个月时,收集远端吻合口和邻近的正常主动脉。取一部分用于组织学检查,并从其余部分中分离总RNA。使用差异mRNA显示来鉴定候选cDNA克隆,与相邻未受影响的主动脉相比,其表达在吻合内膜增生中有所不同。对克隆进行测序,并搜索国家基因数据库。 Northern印迹分析证实了基因表达的改变。结果:筛选出约5000个mRNA种类,获得11个候选克隆。 DNA序列揭示了五个克隆与已知基因序列的同源性。同源基因包括干扰素-γ诱导的人基因(IGUP I-5111),α-1蛋白酶抑制剂基因,人视网膜母细胞瘤易感性基因和人肌酸激酶基因(两个克隆)。 Northern印迹分析显示,在11个中的4个中有4个基因表达改变,在11个中的6个中有无调控信号,在11个中的6个中检测不到信号。发现在内膜增生段中代表IGUP I-5111的克隆的表达降低了三倍以上至仅是正常主动脉中SE水平的31%+/- 16.4%SE。结论:mRNA差异显示技术已在体内吻合内膜增生模型中鉴定出基因表达的差异。在下游的聚四氟乙烯动脉吻合的增生区域内,与干扰素-γ诱导的人类基因同源的RNA的表达持续下降。

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