平滑肌细胞中血管紧张素转换酶mRNA的竞争性缺失突变体定量PCR检测。

PCR methods and applications Pub Date : 1994-12-01 DOI:10.1101/gr.4.3.167

J J Lanzillo, X J Kong, B L Fanburg

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引用次数: 9

摘要

为了定量血管紧张素转换酶(ACE) mRNA，我们开发了一种带有缺失突变内标准的逆转录(RT)偶联竞争性PCR (RT-PCR)测定方法。RT-PCR检测人源和牛源的ACE mRNA。在培养的人隐静脉平滑肌细胞(HuSV-SMCs)和牛肺动脉平滑肌细胞(BPA)的总RNA中检测到ACE mRNA。BPA- smc表达的ACE mRNA比BPA内皮细胞少9倍，比husv - smc少3倍。每微克细胞总RNA中，ACE mRNA的表观量在HuSV-SMCs中为118,350 +/- 2,300拷贝，在BPA-SMCs中为42,200 +/- 11,300拷贝。绝对值的准确性受到用于计算它们的假设的限制。这些数据支持肾素-血管紧张素系统成分由SMCs转录的假设。

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A competitive deletion mutant quantitative PCR assay for angiotensin-converting enzyme mRNA in smooth muscle cells.

To quantify angiotensin-converting enzyme (ACE) mRNA, we have developed a reverse transcription (RT)-coupled competitive PCR (RT-PCR) assay with a deletion mutant internal standard. The RT-PCR detects ACE mRNA from both human and bovine sources. ACE mRNA was detected in total RNA from cultured human saphenous vein smooth muscle cells (HuSV-SMCs) and from bovine pulmonary artery (BPA) SMCs. BPA-SMC expressed ninefold less ACE mRNA than BPA endothelial cells, and threefold less than HuSV-SMCs. Apparent amounts of ACE mRNA were 118,350 +/- 2,300 copies in HuSV-SMCs and 42,200 +/- 11,300 copies in BPA-SMCs per microgram of total cell RNA. The accuracy of the absolute values is subject to the limitations of the assumptions used to calculate them. These data support the hypothesis that components of the renin-angiotensin system are transcribed by SMCs.

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PCR methods and applications

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