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细胞外ATP直接控制兔气道纤毛上皮细胞中的阳离子选择性通道。

Extracellular ATP directly gates a cation-selective channel in rabbit airway ciliated epithelial cells.

作者信息

Korngreen A, Ma W, Priel Z, Silberberg S D

机构信息

Department of Chemistry, Ben-Gurion University of the Negev, Beer-Sheva 84105, Israel.

出版信息

J Physiol. 1998 May 1;508 ( Pt 3)(Pt 3):703-20. doi: 10.1111/j.1469-7793.1998.703bp.x.

Abstract
  1. A membrane conductance activated by extracellular ATP was identified and characterized in freshly dissociated rabbit airway ciliated cells using the whole-cell and outside-out patch configurations of the patch-clamp technique. 2. In solutions designed to maximize currents through voltage-gated calcium channels, there were no indications of voltage-gated Ba2+ currents. 3. Extracellular ATP (but not UTP or ADP) activated a membrane conductance which remained activated for several minutes in the presence of ATP. The conductance was permeable to monovalent and divalent cations with approximate relative permeabilities (P) for PBa : PCs : PTEA of 4 : 1 : 0.1. Permeability to Cl- was negligible. 4. Including GDP-beta-S in the intracellular solution did not inhibit the effects of ATP, nor did GTP-gamma-S irreversibly activate the conductance. 5. In outside-out membrane patches, with GDP-beta-S in the pipette solution, ATP activated ion channels which had a chord conductance of approximately 6 pS in symmetrical 150 mM CsCl solutions at -120 mV. 6. Suramin (100 microM) inhibited the whole-cell currents activated by ATP (200 microM) by 93 +/- 3 %. Similar effects of suramin were observed on ATP-activated channels in outside-out membrane patches. 7. Extracellular ATP had a priming action on the response to subsequent exposure to ATP. At -40 mV, the time to half-maximal current activation (t1/2) was 46 +/- 9 s during the first exposure to 200 microM ATP and decreased to 5 +/- 3 s during a second exposure to the same concentration of ATP. The priming action of ATP was not inhibited by including GDP-beta-S in the intracellular solution. 8. The initial rate of activation increased with the concentration of ATP, and was voltage sensitive. During the first exposure to 200 microM ATP, t1/2 at +40 mV was 4-fold longer than t1/2 at -40 mV. 9. Half-maximal activation of the conductance shifted from 210 +/- 30 to 14 +/- 4 microM added ATP when CaCl2 in the extracellular solution was reduced from 1.58 to 0. 01 mM. The Hill coefficient for ATP was 1.2 in both solutions.10. These observations suggest that a form of ATP uncomplexed with divalent cations directly gates an ion channel (P2X receptor) in rabbit airway ciliated cells, which serves as a pathway for Ca2+ influx. This purinoceptor may contribute to sustained ciliary activation during prolonged exposures to ATP.
摘要
  1. 运用膜片钳技术的全细胞和外向膜片模式,在新鲜分离的兔气道纤毛细胞中识别并表征了一种由细胞外ATP激活的膜电导。2. 在旨在使通过电压门控钙通道的电流最大化的溶液中,未发现电压门控Ba2+电流的迹象。3. 细胞外ATP(而非UTP或ADP)激活了一种膜电导,在ATP存在的情况下,该电导可保持激活状态数分钟。该电导对单价和二价阳离子通透,其相对通透率(P)近似为:PB a:PC s:PTEA = 4:1:0.1。对Cl-的通透性可忽略不计。4. 细胞内溶液中加入GDP-β-S不会抑制ATP的作用,GTP-γ-S也不会不可逆地激活该电导。5. 在外向膜片中,移液管溶液中含有GDP-β-S,在-120 mV的对称150 mM CsCl溶液中,ATP激活了弦电导约为6 pS的离子通道。6. 苏拉明(100 μM)抑制了由ATP(200 μM)激活的全细胞电流的93±3%。在外向膜片中,对ATP激活的通道也观察到了类似的苏拉明效应。7. 细胞外ATP对随后暴露于ATP的反应有引发作用。在-40 mV时,第一次暴露于200 μM ATP期间,电流激活至半最大的时间(t1/2)为46±9秒,第二次暴露于相同浓度的ATP时,t1/2降至5±3秒。细胞内溶液中加入GDP-β-S不会抑制ATP的引发作用。8. 激活的初始速率随ATP浓度增加而增加,且对电压敏感。在第一次暴露于200 μM ATP期间,+40 mV时的t1/2比-40 mV时的长4倍。9. 当细胞外溶液中的CaCl2从1.58 mM降至0.01 mM时,电导激活至半最大时添加的ATP浓度从210±30 μM变为14±4 μM。两种溶液中ATP的希尔系数均为1.2。10. 这些观察结果表明,一种未与二价阳离子结合的ATP形式直接门控兔气道纤毛细胞中的离子通道(P2X受体),该通道是Ca2+内流的途径。这种嘌呤受体可能在长时间暴露于ATP期间有助于持续的纤毛激活。

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