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一种上皮钾通道的一级结构和功能特性

Primary structure and functional properties of an epithelial K channel.

作者信息

Zhou H, Tate S S, Palmer L G

机构信息

Department of Physiology and Biophysics, Cornell University Medical College, New York, New York 10021.

出版信息

Am J Physiol. 1994 Mar;266(3 Pt 1):C809-24. doi: 10.1152/ajpcell.1994.266.3.C809.

Abstract

Expression cloning in Xenopus oocytes was used to identify a clone for a renal K channel. The clone, named ROMK2, was obtained from a cDNA library constructed in the plasmid vector pSPORT using size-selected poly(A)+ RNA from whole rat kidney. ROMK2 consists of 1,837 nucleotides, with an open reading frame of 1,116 bases predicted to code for a 372-amino acid peptide. The clone appears to be a splice variant of a recently reported K channel (ROMK1) from rat renal outer medulla (Ho, K.H., C.G. Nichols, W.J. Lederer, J. Lytton, P.M. Vassilev, M.V. Kanazirska, and S.C. Hebert. Nature Lond. 362: 31-37, 1993). Northern blot analysis indicates that ROMK2 is expressed in renal cortex, medulla, and papilla. Expression in other tissues appears to be much lower. The functional properties of the channel as measured in Xenopus oocytes indicate its close relationship to ROMK1 and more distant relationship to the inward rectifier K channel (IRK1) (Kubo, Y, T.J. Baldwin, Y. N. Jan, and L. Y. Jan. Nature Lond. 362: 127-133, 1993). The inward conductance of the channel is a saturable function of external K, with a half-maximal conductance at <5 mM. The selectivity sequence for ion permeability based on reversal potential measurements was K > Rb > NH4 > Na, Li. The conductance to Rb was only one-half that to K. Extracellular Ba2+ and Cs+ blocked the channel in a voltage-dependent manner. The high sensitivity of Cs+ block to voltage is consistent with the channel's operating as a multi-ion pore. The channel was blocked by high concentrations (100 microM) of glibenclamide. It did not appear to be blocked by extracellular Na+ or tetraethyl-ammonium ion. Patch-clamp measurements indicated a single-channel conductance of 30 pS in the presence of 110 mM K and high open probability that was weakly dependent on voltage. This channel may be involved in maintaining the membrane potential of renal cells and/or mediating renal K secretion.

摘要

利用非洲爪蟾卵母细胞中的表达克隆技术来鉴定一种肾脏钾通道的克隆体。该克隆体名为ROMK2,是从使用来自大鼠全肾的大小选择的聚腺苷酸加尾RNA构建于质粒载体pSPORT中的cDNA文库中获得的。ROMK2由1837个核苷酸组成,具有一个1116个碱基的开放阅读框,预计编码一个372个氨基酸的肽段。该克隆体似乎是最近报道的来自大鼠肾外髓质的钾通道(ROMK1)的剪接变体(Ho,K.H.,C.G. Nichols,W.J. Lederer,J. Lytton,P.M. Vassilev,M.V. Kanazirska,和S.C. Hebert。《自然·伦敦》362:31 - 37,1993)。Northern印迹分析表明ROMK2在肾皮质、髓质和乳头中表达。在其他组织中的表达似乎要低得多。在非洲爪蟾卵母细胞中测量的该通道的功能特性表明它与ROMK1密切相关,而与内向整流钾通道(IRK1)的关系较远(Kubo,Y,T.J. Baldwin,Y.N. Jan,和L.Y. Jan。《自然·伦敦》362:127 - 133,1993)。该通道的内向电导是外部钾的饱和函数,在<5 mM时具有半最大电导。基于反转电位测量的离子通透性选择性序列为K > Rb > NH4 > Na,Li。对Rb的电导仅为对K的电导的一半。细胞外Ba2+和Cs+以电压依赖性方式阻断该通道。Cs+阻断对电压的高敏感性与该通道作为多离子孔起作用一致。该通道被高浓度(100 microM)的格列本脲阻断。它似乎不被细胞外Na+或四乙铵离子阻断。膜片钳测量表明在存在110 mM K时单通道电导为30 pS,且开放概率高,对电压的依赖性较弱。该通道可能参与维持肾细胞的膜电位和/或介导肾脏钾分泌。

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