Terris J M, Knepper M A, Wade J B
Laboratory of Kidney and Electrolyte Metabolism, National Heart, Lung, and Blood Institute, National Institutes of Health, Bethesda, Maryland 21201, USA.
Am J Physiol Renal Physiol. 2001 Feb;280(2):F325-32. doi: 10.1152/ajprenal.2001.280.2.F325.
UT-A3 has recently been identified as a splicing variant transcript of the UT-A gene present in the kidney. To study the cellular and subcellular localization of UT-A3, we raised a new polyclonal antibody to its COOH-terminal end. Immunoblots identified bands at 44 and 67 kDa predominately in the inner medulla and showed that the antibody does not recognize UT-A1. Deglycosylation with PNGase decreased the molecular mass of both forms to 40 kDa. UT-A3 is most abundant in the inner third of the inner medulla and is present in membrane fractions. Cell fractionation studies showed that UT-A3 is only detectable in inner medullary collecting duct (IMCD) cells. These observations were confirmed with immunolocalization studies demonstrating an exclusive labeling of IMCD cells. Double-labeling studies with anti-Na-K-ATPase demonstrated UT-A3 in intracellular membranes and in the apical region but were incompatible with a basolateral site for UT-A3. Although the function of this isoform in the inner medulla is unknown, the large abundance suggests that it may be important in the renal handling of urea.
UT - A3最近被鉴定为存在于肾脏中的UT - A基因的一种剪接变异转录本。为了研究UT - A3的细胞和亚细胞定位,我们针对其COOH末端制备了一种新的多克隆抗体。免疫印迹在44 kDa和67 kDa处鉴定出条带,主要位于髓质内层,并且表明该抗体不识别UT - A1。用PNGase进行去糖基化处理后,两种形式的分子量均降至40 kDa。UT - A3在髓质内层的内三分之一区域最为丰富,并且存在于膜组分中。细胞分级分离研究表明,UT - A3仅在内髓集合管(IMCD)细胞中可检测到。这些观察结果通过免疫定位研究得到证实,显示IMCD细胞有特异性标记。用抗钠钾ATP酶进行双重标记研究表明,UT - A3存在于细胞内膜和顶端区域,但与UT - A3位于基底外侧位点不相符。尽管这种异构体在髓质内层的功能尚不清楚,但大量存在表明它可能在肾脏对尿素的处理中起重要作用。
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