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首页> 外文期刊>The Journal of biological chemistry >WATER AND GLYCEROL PERMEABILITIES OF AQUAPORINS 1-5 AND MIP DETERMINED QUANTITATIVELY BY EXPRESSION OF EPITOPE-TAGGED CONSTRUCTS IN XENOPUS OOCYTES
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WATER AND GLYCEROL PERMEABILITIES OF AQUAPORINS 1-5 AND MIP DETERMINED QUANTITATIVELY BY EXPRESSION OF EPITOPE-TAGGED CONSTRUCTS IN XENOPUS OOCYTES

机译:水通道蛋白 1-5 和 MIP 的水和甘油通透性通过非洲爪蟾卵母细胞中表位标记构建体的表达定量确定

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The goal of this study was to compare single channel water and glycerol permeabilities of mammalian aqua-porins (AQP) 1-5 and the major intrinsic protein of lens fiber (MIP). Each of the six cloned cDNAs from rat was left untagged or was epitope-tagged with c-Myc or FLAG at either the N or C terminus so that results would not depend on epitope identity or location. The constructs were expressed in Xenopus oocytes for measurement of osmotic water permeability (P-f), H-3glycerol uptake, and protein expression. Each of the 30 epitope-tagged constructs was expressed strongly at the oocyte plasma membrane. The 10-min uptake of H-3glycerol was increased significantly (range of 4.5-8-fold over control) in oocytes expressing untagged AQP3 (GLIP) and each of the four tagged AQP3 constructs; H-3glycerol uptake was not increased in oocytes expressing AQP1, AQP2, AQP4, AQP5, or MIP. In oocytes microinjected with 5 ng of cRNA, average P-f values (in cm/s x 10(-3)) were 0.67 +/- 0.06 (control), 19 +/- 2 (AQP1), 10 +/- 1 (AQP2), 8 +/- 2 (AQP3), 29 +/- 1 (AQP4), 10 +/- 1 (AQP5), and 1.3 +/- 0.2 (MIP), and they were relatively insensitive to the presence, identity, or location of the epitope tag. P-f values were not affected by protein kinase A or C activation. After normalization for plasma membrane expression by immunoprecipitation of microdissected plasma membranes, single channel water permeabilities (p(f), referenced to the AQP1 p(f) of 6 x 10(-14) cm(3)/s) were (in cm(3)/s x 10(-14)) 3.3 +/- 0.2 (AQP2), 2.1 +/- 0.3 (AQP3), 24 +/- 0.6 (AQP4), 5.0 +/- 0.4 (AQP5), and 0.25 +/- 0.05 (MIP); p(f) values were insensitive to epitope identity and location. These results indicate very different intrinsic water permeabilities for the mammalian aquaporin homologs, with the p(f) value for AQP4 remarkably higher than those for the others. The p(f) values establish limits on aquaporin tissue densities required for physiological function and suggest significant structural and functional differences among the aquaporins. References: 55
机译:本研究的目的是比较哺乳动物水孔蛋白 (AQP) 1-5 和晶状体纤维主要内在蛋白 (MIP) 的单通道水和甘油通透性。来自大鼠的六种克隆cDNA中的每一个都没有标记,或者在N或C末端用c-Myc或FLAG标记表位,因此结果不依赖于表位身份或位置。这些构建体在非洲爪蟾卵母细胞中表达,用于测量渗透性透水性 (P-f)、[H-3] 甘油摄取和蛋白质表达。30 个表位标记的构建体中的每个都在卵母细胞质膜上强烈表达。在表达未标记 AQP3 (GLIP) 的卵母细胞和四种标记的 AQP3 构建体中,[H-3] 甘油的 10 分钟摄取显着增加(范围为对照组的 4.5-8 倍);在表达 AQP1、AQP2、AQP4、AQP5 或 MIP 的卵母细胞中,[H-3]甘油摄取量未增加。在显微注射 5 ng cRNA 的卵母细胞中,平均 P-f 值(以 cm/s x 10(-3)为单位)为 0.67 +/- 0.06(对照)、19 +/- 2 (AQP1)、10 +/- 1 (AQP2)、8 +/- 2 (AQP3)、29 +/- 1 (AQP4)、10 +/- 1 (AQP5) 和 1.3 +/- 0.2 (MIP),并且它们对表位标签的存在、身份或位置相对不敏感。P-f值不受蛋白激酶A或C激活的影响。通过对显微解剖质膜进行免疫沉淀对质膜表达进行标准化后,单通道透水性 (p(f),参考 6 x 10(-14) cm(3)/s) 的 AQP1 p(f) 为 (cm(3)/s x 10(-14)) 3.3 +/- 0.2 (AQP2)、2.1 +/- 0.3 (AQP3)、24 +/- 0.6 (AQP4)、5.0 +/- 0.4 (AQP5) 和 0.25 +/- 0.05 (MIP);P(F)值对表位身份和位置不敏感。这些结果表明,哺乳动物水通道蛋白同系物的内在透水性非常不同,AQP4的p(f)值明显高于其他同源物。p(f)值建立了生理功能所需的水通道蛋白组织密度的限制,并表明水通道蛋白之间的结构和功能存在显着差异。[参考文献: 55]

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