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环磷酸腺苷核糖,一种假定的可动员钙离子的第二信使,在黏膜下腺泡细胞中发挥作用。

Cyclic ADP-ribose, a putative Ca2+-mobilizing second messenger, operates in submucosal gland acinar cells.

作者信息

Sasamori Kan, Sasaki Tsukasa, Takasawa Shin, Tamada Tsutomu, Nara Masayuki, Irokawa Toshiya, Shimura Sanae, Shirato Kunio, Hattori Toshio

机构信息

Division of Respiratory and Infectious Diseases, Tohoku University Graduate School of Medicine, Sendai, Japan.

出版信息

Am J Physiol Lung Cell Mol Physiol. 2004 Jul;287(1):L69-78. doi: 10.1152/ajplung.00454.2003. Epub 2004 Feb 27.

DOI:10.1152/ajplung.00454.2003
PMID:14990397
Abstract

Cyclic ADP-ribose (cADPR), a putative Ca(2+)-mobilizing second messenger, has been reported to operate in several mammalian cells. To investigate whether cADPR is involved in electrolyte secretion from airway glands, we used a patch-clamp technique, the measurement of microsomal Ca(2+) release, quantification of cellular cADPR, and RT-PCR for CD38 mRNA in human and feline tracheal glands. cADPR (>6 microM), infused into the cell via the patch pipette, caused ionic currents dependent on cellular Ca(2+). Infusions of lower concentrations (2-4 microM) of cADPR or inositol 1,4,5-trisphosphate (IP(3)) alone were without effect on the baseline current, but a combined application of cADPR and IP(3) mimicked the cellular response to low concentrations of acetylcholine (ACh). Microsomes derived from the isolated glands released Ca(2+) in response to both IP(3) and cADPR. cADPR released Ca(2+) from microsomes desensitized to IP(3) or those treated with heparin. The mRNA for CD38, an enzyme protein involved in cADPR metabolism, was detected in human tissues, including tracheal glands, and the cellular content of cADPR was increased with physiologically relevant concentrations of ACh. We conclude that cADPR, in concert with IP(3), operates in airway gland acinar cells to mobilize Ca(2+), resulting in Cl(-) secretion.

摘要

环磷酸腺苷核糖(cADPR)是一种被认为可动员钙离子的第二信使,据报道其在多种哺乳动物细胞中发挥作用。为了研究cADPR是否参与气道腺体的电解质分泌,我们采用了膜片钳技术、微粒体钙离子释放测量、细胞内cADPR定量以及人及猫气管腺体中CD38 mRNA的逆转录聚合酶链反应(RT-PCR)。通过膜片吸管将cADPR(>6 microM)注入细胞,可引起依赖细胞内钙离子的离子电流。单独注入较低浓度(2 - 4 microM)的cADPR或肌醇1,4,5 - 三磷酸(IP(3))对基线电流无影响,但联合应用cADPR和IP(3)可模拟细胞对低浓度乙酰胆碱(ACh)的反应。从分离腺体获得的微粒体对IP(3)和cADPR均有钙离子释放反应。cADPR可从对IP(3)脱敏或经肝素处理的微粒体中释放钙离子。在包括气管腺体在内的人体组织中检测到了参与cADPR代谢的酶蛋白CD38的mRNA,并且细胞内cADPR的含量随生理相关浓度的ACh而增加。我们得出结论,cADPR与IP(3)协同作用于气道腺泡细胞,动员钙离子,从而导致氯离子分泌。

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