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实时测量活体粘菌细胞中环腺苷酸(cAMP)的产生。

Real-time measurements of cAMP production in live Dictyostelium cells.

机构信息

Laboratory of Cellular and Molecular Biology, Center for Cancer Research, National Cancer Institute, National Institutes of Health, Bethesda, MD 20892, USA.

出版信息

J Cell Sci. 2009 Nov 1;122(Pt 21):3907-14. doi: 10.1242/jcs.051987. Epub 2009 Oct 6.

Abstract

Cyclic AMP has a crucial role during the entire developmental program of the social amoebae Dictyostelium, acting both as an intracellular second messenger and, when secreted, as a directional cue that is relayed to neighboring cells during chemotaxis. Although significant knowledge about cAMP production in chemotaxing cells has been derived from studies performed on cell populations, cAMP dynamics at the single cell level have not been investigated. To examine this, we used a FRET-based cAMP sensor that possesses high cAMP sensitivity and great temporal resolution. We show the transient profile of cAMP accumulation in live Dictyostelium cells and establish that chemoattractants control intracellular cAMP dynamics by regulating synthesis via the adenylyl cyclase ACA. aca(-) cells show no significant change in FRET response following chemoattractant addition. Furthermore, cells lacking ACB, the other adenylyl cyclase expressed in chemotaxing cells, behave similarly to wild-type cells. We also establish that the RegA is the major phosphodiesterase that degrades intracellular cAMP in chemotaxis-competent cells. Interestingly, we failed to measure intracellular cAMP compartmentalization in actively chemotaxing cells. We conclude that cytosolic cAMP, which is destined to activate PKA, is regulated by ACA and RegA and does not compartmentalize during chemotaxis.

摘要

环腺苷酸(cAMP)在社会性粘菌 Dictyostelium 的整个发育程序中起着至关重要的作用,它既是细胞内的第二信使,又是一种趋化性过程中分泌的定向信号,可以被传递到相邻细胞。虽然已经从细胞群体的研究中获得了关于趋化细胞中 cAMP 产生的大量知识,但尚未研究单细胞水平的 cAMP 动力学。为了研究这一点,我们使用了一种基于 FRET 的 cAMP 传感器,它具有高 cAMP 灵敏度和很好的时间分辨率。我们展示了活 Dictyostelium 细胞中 cAMP 积累的瞬态分布,并确定趋化剂通过调节腺苷酸环化酶 ACA 的合成来控制细胞内的 cAMP 动力学。aca(-)细胞在添加趋化剂后,FRET 反应没有明显变化。此外,缺乏在趋化性细胞中表达的另一种腺苷酸环化酶 ACB 的细胞表现出与野生型细胞相似的行为。我们还确定 RegA 是在有趋化性能力的细胞中降解细胞内 cAMP 的主要磷酸二酯酶。有趣的是,我们未能在活跃的趋化性细胞中测量细胞内 cAMP 的区室化。我们的结论是,cAMP 是细胞内 PKA 的激活剂,它由 ACA 和 RegA 调节,在趋化性过程中不进行区室化。

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