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拉伸可增加气道上皮细胞中肌醇1,4,5 -三磷酸的浓度。

Stretch increases inositol 1,4,5-trisphosphate concentration in airway epithelial cells.

作者信息

Felix J A, Woodruff M L, Dirksen E R

机构信息

Department of Neurobiology, UCLA School of Medicine, Los Angeles, California, USA.

出版信息

Am J Respir Cell Mol Biol. 1996 Mar;14(3):296-301. doi: 10.1165/ajrcmb.14.3.8845181.

Abstract

Mechanical stimulation of airway epithelial cells with a microprobe leads to an increase in cytoplasmic [Ca2+] that appears to be due, in part, to release of Ca2+ from inositol 1,4,5-trisphosphate (IP3)-sensitive stores (Boitano et al., Science 258:292[1992]). To investigate whether intracellular IP3 concentration ([IP3]i) increases in response to mechanical stimulation, we grew confluent monolayers from rabbit tracheal mucosal explants on flexible substrates and measured [IP3]i after stretching the substrate. The effect of stretch on [IP3]i was measured in the presence of Li+, an inhibitor of IP3 degradation. In unstretched cells, IP3 measured approximately 5.1 pmol/10(6) cells, from which we estimated [IP3]i to be 1.8 microM. Addition of Li+ had no effect on resting [IP3]i. When the flexible cell support was stretched to increase its surface area by 13%, mean [IP3]i increased about 3-fold with a half-time of approximately 1 s. The increased [IP3]i was maintained in a plateau phase for approximately 8 s and then decayed to near the unstretched level over the next 10 s, despite the sustained application of stretch. A transient stretch (0.5 s) induced a similar rate of increase and peak [IP3]i; however, [IP3]i subsided without a plateau phase. The magnitude of the [IP3]i increase was proportional to stimulus intensity between 0 and 13% increase in substrate surface area. In addition, dissociated airway epithelial cells were exposed to hypotonic solution to induce cell swelling. [IP3]i increased about 4-fold above control levels after 10 s of exposure to hypotonic solution. Basal [IP3]i of dissociated cells in isotonic solution was estimated to be 0.7 microM. These results are consistent with mechanical stimulation leading to phospholipase C synthesis of IP3, which mediates intracellular and intercellular Ca2+ signaling.

摘要

用微探针机械刺激气道上皮细胞会导致细胞质中[Ca2+]增加,这似乎部分归因于肌醇1,4,5 -三磷酸(IP3)敏感储存库中Ca2+的释放(博伊塔诺等人,《科学》258:292[1992])。为了研究细胞内IP3浓度([IP3]i)是否会因机械刺激而增加,我们在柔性基质上培养了来自兔气管黏膜外植体的汇合单层细胞,并在拉伸基质后测量[IP3]i。在存在IP3降解抑制剂Li+的情况下测量拉伸对[IP3]i的影响。在未拉伸的细胞中,IP3约为5.1 pmol/10(6)个细胞,据此我们估计[IP3]i为1.8 microM。添加Li+对静息[IP3]i无影响。当柔性细胞支持物被拉伸以使其表面积增加13%时,平均[IP3]i增加约3倍,半衰期约为1秒。增加的[IP3]i在平台期维持约8秒,然后在接下来的10秒内衰减至接近未拉伸水平,尽管持续施加拉伸。短暂拉伸(0.5秒)诱导了类似的增加速率和[IP3]i峰值;然而,[IP3]i没有平台期就下降了。在基质表面积增加0至13%之间,[IP3]i增加的幅度与刺激强度成正比。此外,将分离的气道上皮细胞暴露于低渗溶液中以诱导细胞肿胀。暴露于低渗溶液10秒后,[IP3]i比对照水平增加约4倍。等渗溶液中分离细胞的基础[IP3]i估计为0.7 microM。这些结果与机械刺激导致IP3的磷脂酶C合成一致,IP3介导细胞内和细胞间Ca2+信号传导。

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