Meier Stuart K, Donald John A
School of Biological and Chemical Sciences, Deakin University, Geelong, Victoria, 3217, Australia.
Gen Comp Endocrinol. 2002 Feb 1;125(2):207-17. doi: 10.1006/gcen.2001.7761.
This study aimed to localize and characterize natriuretic peptide binding sites in the urinary bladder of Bufo marinus and to then examine the effect of natriuretic peptides on the bladder vascular tone and water reabsorption in isolated perfused bladder preparations. Specific (125)I-rat atrial natriuretic peptide ((125)I-rANP) binding sites were present on blood vessels, muscle, and epithelium. In tissue sections and/or isolated membranes, the binding was completely displaced by frog ANP, rat ANP, and porcine C-type natriuretic peptide (CNP; membranes only). However, a reduction in binding was observed after incubation with (125)I-rANP and 1 microM of the natriuretic peptide receptor-C (NPR-C) ligand C-ANF, but residual binding remained suggesting the presence of two distinct binding sites. Electrophoresis of bladder membranes cross-linked to (125)I-rANP identified two bands at approximately 70 and 140 kDa that correspond to the monomeric mass of NPR-C and the guanylate cyclase receptors, respectively. Furthermore, the presence of natriuretic peptide receptor-A and NPR-C mRNA in the bladder was demonstrated with reverse transcription--polymerase chain reaction. In addition, rat ANP, frog ANP, and porcine CNP stimulated a significant increase in cGMP generation in bladder membrane preparations, which indicated the presence of guanylate cyclase-linked receptors. In perfused bladder preparations, arginine vasotocin increased perfusion pressure and water permeability. The infusion of frog ANP or porcine CNP failed to alter perfusion pressure or water reabsorption in the presence or absence of arginine vasotocin. This study identified a well-developed natriuretic peptide receptor system in the urinary bladder of B. marinus but the function of the receptors remains unclear.
本研究旨在定位并表征海蟾蜍膀胱中的利钠肽结合位点,进而研究利钠肽对离体灌注膀胱标本中膀胱血管张力和水重吸收的影响。特异性的(125)I-大鼠心房利钠肽((125)I-rANP)结合位点存在于血管、肌肉和上皮组织中。在组织切片和/或分离的膜中,该结合可被蛙心房利钠肽、大鼠心房利钠肽和猪C型利钠肽(仅在膜中)完全取代。然而,在与(125)I-rANP和1微摩尔的利钠肽受体-C(NPR-C)配体C-ANF孵育后,结合有所减少,但仍有残留结合,提示存在两种不同的结合位点。与(125)I-rANP交联的膀胱膜电泳鉴定出两条分别约为70 kDa和140 kDa的条带,它们分别对应于NPR-C的单体质量和鸟苷酸环化酶受体。此外,通过逆转录-聚合酶链反应证实膀胱中存在利钠肽受体-A和NPR-C mRNA。另外,大鼠心房利钠肽、蛙心房利钠肽和猪C型利钠肽可刺激膀胱膜制剂中cGMP生成显著增加,这表明存在与鸟苷酸环化酶相连的受体。在灌注膀胱标本中,精氨酸血管催产素可增加灌注压力和水通透性。无论有无精氨酸血管催产素,输注蛙心房利钠肽或猪C型利钠肽均未能改变灌注压力或水重吸收。本研究在海蟾蜍膀胱中鉴定出一个发育完善的利钠肽受体系统,但这些受体的功能仍不清楚。