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机械加载的猪软骨细胞团在微团培养中释放三磷酸腺苷

ATP release by mechanically loaded porcine chondrons in pellet culture.

作者信息

Graff R D, Lazarowski E R, Banes A J, Lee G M

机构信息

The University of North Carolina at Chapel Hill, 27599-7280, USA.

出版信息

Arthritis Rheum. 2000 Jul;43(7):1571-9. doi: 10.1002/1529-0131(200007)43:7<1571::AID-ANR22>3.0.CO;2-L.

Abstract

OBJECTIVE

To determine whether ATP is released from chondrocytes during mechanical stimulation and whether degradation of ATP generates inorganic pyrophosphate in chondron pellet cultures.

METHODS

Chondron pellets were formed from 1.6 x 10(6) cells that had been enzymatically isolated from porcine articular cartilage. ATP was measured in media from cultures at rest and during fluid movement and cyclic compression. ATP hydrolysis was examined by high-performance liquid chromatography following the addition of gamma32P-ATP to resting cultures.

RESULTS

Pellet cultures at rest maintained a steady-state concentration of 2-4 nM ATP in 2 ml of medium. The ATP concentration increased 5-12-fold with cyclic compression (7.5 and 15 kPa at 0.5 Hz), then decreased to preloading levels within 60 minutes despite continued loading. A subsequent increase in pressure stimulated a further increase in ATP release, suggesting that chondrocytes desensitize to load. Cell viability was similar for pellets at rest and up to 24 hours after compression. ATP released in response to mechanical stimulation was inhibited 50% by 0.5 mM octanol, suggesting a regulated mechanism for ATP release. Exogenous ATP was rapidly hydrolyzed to pyrophosphate in resting cultures.

CONCLUSION

The occurrence of basal levels of extracellular ATP in the presence of pyrophosphohydrolase activity indicates that ATP was continuously released by chondrocytes at rest. Considering that chondrocytes express purinoceptors that respond to ATP, we suggest a role for ATP in extracellular signaling by chondrocytes in response to mechanical load. ATP released by chondrocytes in response to mechanical load is a likely source of pyrophosphate in calcium pyrophosphate dihydrate crystal deposition diseases.

摘要

目的

确定在机械刺激过程中软骨细胞是否释放三磷酸腺苷(ATP),以及在软骨粒培养物中ATP的降解是否会生成无机焦磷酸。

方法

从猪关节软骨酶解分离出的1.6×10⁶个细胞形成软骨粒。在静止培养以及液体流动和循环压缩过程中,测量培养基中的ATP。在静止培养物中加入γ³²P-ATP后,通过高效液相色谱法检测ATP水解情况。

结果

静止的软骨粒培养物在2ml培养基中维持2 - 4nM ATP的稳态浓度。随着循环压缩(0.5Hz下7.5和15kPa),ATP浓度增加5 - 12倍,然后尽管持续加载,在60分钟内降至预加载水平。随后压力增加刺激ATP释放进一步增加,表明软骨细胞对负荷脱敏。静止和压缩后长达24小时的软骨粒细胞活力相似。0.5mM辛醇可抑制机械刺激释放的ATP的50%,表明ATP释放存在调节机制。在静止培养物中,外源性ATP迅速水解为焦磷酸。

结论

在焦磷酸水解酶活性存在的情况下,细胞外ATP基础水平的出现表明静止的软骨细胞持续释放ATP。鉴于软骨细胞表达对ATP有反应的嘌呤受体,我们认为ATP在软骨细胞响应机械负荷的细胞外信号传导中起作用。软骨细胞响应机械负荷释放的ATP可能是二水焦磷酸钙晶体沉积疾病中焦磷酸的来源。

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