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绵羊瘤胃上皮中的碳酸氢盐输出转运体

Bicarbonate exporting transporters in the ovine ruminal epithelium.

作者信息

Bilk S, Huhn K, Honscha K U, Pfannkuche H, Gäbel G

机构信息

Institute of Veterinary-Physiology, Leipzig University, An den Tierkliniken 7, 04103 Leipzig, Germany.

出版信息

J Comp Physiol B. 2005 Jul;175(5):365-74. doi: 10.1007/s00360-005-0493-1. Epub 2005 May 31.

Abstract

In order to stabilize the intraruminal pH, bicarbonate secretion by the ruminal epithelium seems to be an important prerequisite. The present study therefore focussed on the characterization of bicarbonate exporting systems in ruminal epithelial cells. Intracellular pH (pH(i)) was measured spectrofluorometrically in primary cultured ruminal epithelial cells loaded with the pH-sensitive fluorescent dye, 2,7-bis(carboxyethyl)-5(6')-carboxyfluorescein acetomethyl ester. Switching from CO2/HCO3- -buffered to HEPES-buffered solution caused a rapid intracellular alkalinization followed by a counter-regulation towards initial pH(i). The recovery of pH(i) was dependent upon extracellular chloride, but independent of extracellular sodium. Adding 500 microM H2DIDS significantly reduced the increase of pH(i). For further characterization of the bicarbonate exporting systems, we tested the ability to reverse the direction from HCO3- export to import in the absence of sodium and chloride. Under sodium and chloride-free conditions, counter-regulation after CO2-induced pH(i) decrease did not differ from pH(i) recovery in the presence of sodium and chloride. Existence of bicarbonate exporting systems in cultured ruminal epithelial cells and intact ruminal epithelium was verified by reverse transcription polymerase chain reaction (RT-PCR). Using RT-PCR and subsequent sequencing, expression of mRNA encoding for AE2, DRA and PAT1 could be found. Bicarbonate exporting systems could therefore be detected both on the functional and structural level.

摘要

为了稳定瘤胃内的pH值,瘤胃上皮分泌碳酸氢盐似乎是一个重要的前提条件。因此,本研究聚焦于瘤胃上皮细胞中碳酸氢盐输出系统的特性研究。在原代培养的瘤胃上皮细胞中,使用对pH敏感的荧光染料2,7-双(羧乙基)-5(6')-羧基荧光素乙酰甲酯,通过荧光分光光度法测量细胞内pH值(pH(i))。从CO2/HCO3-缓冲溶液切换到HEPES缓冲溶液会导致细胞内迅速碱化,随后朝着初始pH(i)进行反向调节。pH(i)的恢复依赖于细胞外氯离子,但与细胞外钠离子无关。添加500 microM H2DIDS可显著降低pH(i)的升高。为了进一步表征碳酸氢盐输出系统,我们测试了在无钠和无氯条件下将HCO3-输出方向逆转至输入方向的能力。在无钠和无氯条件下,CO2诱导的pH(i)降低后的反向调节与存在钠和氯时的pH(i)恢复没有差异。通过逆转录聚合酶链反应(RT-PCR)验证了培养的瘤胃上皮细胞和完整瘤胃上皮中存在碳酸氢盐输出系统。使用RT-PCR及后续测序,可发现编码AE2、DRA和PAT1的mRNA表达。因此,在功能和结构层面均检测到了碳酸氢盐输出系统。

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