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大鼠肾脏含有高水平的促尿钠排泄肽原(尿钠肽原前体),但不表达 GC-C(肠源尿钠肽受体)。

The rat kidney contains high levels of prouroguanylin (the uroguanylin precursor) but does not express GC-C (the enteric uroguanylin receptor).

机构信息

Department of Cell and Molecular Physiology, University of North Carolina, Chapel Hill, NC 27599-7545, USA.

出版信息

Am J Physiol Renal Physiol. 2011 Feb;300(2):F561-73. doi: 10.1152/ajprenal.00282.2010. Epub 2010 Nov 24.

Abstract

The peptide uroguanylin (Ugn) regulates enteric and renal electrolyte transport. Previous studies have shown that Ugn and its receptor GC-C (a ligand-activated guanylate cyclase) are abundant in the intestine. Less is known about Ugn and GC-C expression in the kidney. Here, we identify a 9.4-kDa polypeptide in rat kidney extracts that appears, based on its biochemical and immunological properties, to be authentic prouroguanylin (proUgn). This propeptide is relatively plentiful in the kidney (~16% of intestinal levels), whereas its mRNA is marginally present (<1% of intestinal levels), and free Ugn peptide levels are below detection limits (<0.4% of renal proUgn levels). The paucity of preproUgn-encoding mRNA and free Ugn peptide raises the possibility that the kidney might absorb intact proUgn from plasma, where the concentration of propeptide greatly exceeds that of Ugn. However, immunocytochemical analysis reveals that renal proUgn is found exclusively in distal tubular segments, sites previously shown not to accumulate radiolabeled proUgn after intravascular infusions. Thus proUgn appears to be synthesized within the kidney, but the factors that determine its abundance (rates of transcription, translation, processing, and secretion) must be balanced quite differently than in the gut. Surprisingly, we also find negligible expression of GC-C in the rat kidney, a result confirmed both by RT-PCR and by functional assays that measure Ugn-activated cGMP synthesis. Taken together, these data provide evidence for an intrarenal Ugn system that differs from the well-described intestinal system in its regulatory mechanisms and in the receptor targeted by the peptide.

摘要

尿鸟苷素(Ugn)调节肠道和肾脏电解质转运。先前的研究表明,尿鸟苷素及其受体 GC-C(一种配体激活的鸟苷酸环化酶)在肠道中丰富。关于肾脏中尿鸟苷素和 GC-C 的表达知之甚少。在这里,我们在大鼠肾提取物中鉴定出一种 9.4 kDa 的多肽,根据其生化和免疫学特性,该多肽似乎是真正的尿鸟苷素前体(proUgn)。这种前肽在肾脏中相对丰富(~肠道水平的 16%),而其 mRNA 仅微量存在(<肠道水平的 1%),游离尿鸟苷素肽水平低于检测限(<肾 proUgn 水平的 0.4%)。前尿鸟苷素编码 mRNA 和游离尿鸟苷素肽的缺乏使得肾脏可能从血浆中吸收完整的 proUgn 的可能性增加,其中前肽的浓度大大超过 Ugn 的浓度。然而,免疫细胞化学分析显示,肾脏 proUgn 仅存在于远曲小管段,这些部位先前在血管内输注后未发现放射性标记的 proUgn 积累。因此,proUgn 似乎在肾脏内合成,但决定其丰度的因素(转录、翻译、加工和分泌的速率)必须与肠道中的情况非常不同。令人惊讶的是,我们还发现大鼠肾脏中 GC-C 的表达可忽略不计,这一结果通过 RT-PCR 和功能性测定证实,这些测定测量 Ugn 激活的 cGMP 合成。综上所述,这些数据为肾脏内的 Ugn 系统提供了证据,该系统在其调节机制和肽靶向的受体方面与已描述的肠道系统不同。

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