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微切割大鼠肾单位各节段中的腺苷A1受体信使核糖核酸

Adenosine A1 receptor mRNA in microdissected rat nephron segments.

作者信息

Yamaguchi S, Umemura S, Tamura K, Iwamoto T, Nyui N, Ishigami T, Ishii M

机构信息

Second Department of Internal Medicine, Yokohama City University School of Medicine, Japan.

出版信息

Hypertension. 1995 Dec;26(6 Pt 2):1181-5. doi: 10.1161/01.hyp.26.6.1181.

DOI:10.1161/01.hyp.26.6.1181
PMID:7498992
Abstract

Adenosine plays several roles in the kidney mediated by the specific receptors A1, A2, and possibly A3. We studied the localization of adenosine A1 receptor mRNA in rat nephron segments using reverse transcription and polymerase chain reaction (RT-PCR). The nephron segments of male Sprague-Dawley rats (6 to 8 weeks old) were microdissected. Total RNA was prepared by the acid-guanidinium-phenol-chloroform method and used in the following RT-PCR assay. Because the PCR primers spanned no intron, samples reacted in the absence of RT were used as controls for amplification of genomic DNA. The PCR products were size-fractionated by electrophoresis, visualized with ethidium bromide staining, and confirmed by Southern blot analysis. PCR products were detected in all of the nephron segments examined. No signals were detected in samples reacted in the absence of RT. Strong signals were detected in glomeruli, medullary collecting duct, cortical thick ascending limb, and medullary thick ascending limb, while weak signals were found in proximal convoluted and straight tubules. Previously, the presence of A1 receptors has been demonstrated in glomeruli, collecting duct, and thick ascending limb in the rat kidney by autoradiography and binding studies. In addition to these segments, we further detected A1 receptor mRNA in proximal convoluted and straight tubules. Thus, A1 receptor mRNA seems to be broadly expressed along the nephron.

摘要

腺苷通过特定的A1、A2以及可能的A3受体在肾脏中发挥多种作用。我们使用逆转录聚合酶链反应(RT-PCR)研究了大鼠肾单位各节段中腺苷A1受体mRNA的定位。对雄性Sprague-Dawley大鼠(6至8周龄)的肾单位各节段进行显微解剖。采用酸胍-酚-氯仿法制备总RNA,并用于后续的RT-PCR检测。由于PCR引物不跨越内含子,未进行逆转录反应的样本用作基因组DNA扩增的对照。PCR产物通过电泳进行大小分级,用溴化乙锭染色可视化,并通过Southern印迹分析进行确认。在所检测的所有肾单位节段中均检测到PCR产物。在未进行逆转录反应的样本中未检测到信号。在肾小球、髓质集合管、皮质厚升支和髓质厚升支中检测到强信号,而在近端曲管和直小管中发现弱信号。此前,通过放射自显影和结合研究已证实大鼠肾脏的肾小球、集合管和厚升支中存在A1受体。除了这些节段外,我们还在近端曲管和直小管中进一步检测到了A1受体mRNA。因此,A1受体mRNA似乎在整个肾单位中广泛表达。

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