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调控小鼠的光生物节律反应:Id2-/- 小鼠生物钟系统的不同反应取决于昼夜相位以及光照的时长和强度。

Regulates Photic Entrainment Responses in Mice: Differential Responses of the Id2-/- Mouse Circadian System Are Dependent on Circadian Phase and on Duration and Intensity of Light.

机构信息

Department of Biological Sciences, Galvin Life Science Center, University of Notre Dame, Notre Dame, Indiana.

Eck Institute for Global Health, University of Notre Dame, Notre Dame, Indiana.

出版信息

J Biol Rhythms. 2020 Dec;35(6):555-575. doi: 10.1177/0748730420957504. Epub 2020 Sep 28.

Abstract

ID2 is a rhythmically expressed helix-loop-helix transcriptional repressor, and its deletion results in abnormal properties of photoentrainment. By examining parametric and nonparametric models of entrainment, we have started to explore the mechanism underlying this circadian phenotype. -/- mice were exposed to differing photoperiods, and the phase angle of entrainment under short days was delayed 2 h as compared with controls. When exposed to long durations of continuous light, enhanced entrainment responses were observed after a delay of the clock but not with phase advances. However, the magnitude of phase shifts was not different in -/- mice tested in constant darkness using a discrete pulse of saturating light. No differences were observed in the speed of clock resetting when challenged by a series of discrete pulses interspaced by varying time intervals. A photic phase-response curve was constructed, although no genotypic differences were observed. Although phase shifts produced by discrete saturating light pulses at CT16 were similar, treatment with a subsaturating pulse revealed a ~2-fold increase in the magnitude of the -/- shift. A corresponding elevation of light-induced expression was observed in the -/- suprachiasmatic nucleus (SCN). To test whether the phenotype is based on a sensitivity change at the level of the retina, pupil constriction responses were measured. No differences were observed in responses or in retinal histology, suggesting that the phenotype occurs downstream of the retina and retinal hypothalamic tract. To test whether the phenotype is due to a reduced amplitude of state variables of the clock, the expression of clock genes and was assessed in vivo and in SCN tissue explants. Amplitude, phase, and period length were normal in -/- mice. These findings suggest that ID2 contributes to a photoregulatory mechanism at the level of the SCN central pacemaker through control of the photic induction of negative elements of the clock.

摘要

ID2 是一个节律表达的螺旋-环-螺旋转录因子抑制物,其缺失导致光驯化异常。通过检查驯化的参数和非参数模型,我们开始探索这种生物钟表型的机制。/- 小鼠暴露于不同的光周期下,在短日下的驯化相位角延迟了 2 小时,与对照组相比。当暴露于长时间的连续光照下时,观察到时钟延迟后增强的驯化反应,但没有相位提前。然而,在使用饱和光离散脉冲在持续黑暗中测试的 -/- 小鼠中,相位偏移的幅度没有差异。在受到一系列离散脉冲刺激时,时钟重置的速度没有差异,这些脉冲之间间隔不同的时间。构建了光相反应曲线,尽管没有观察到基因型差异。尽管 CT16 时离散饱和光脉冲产生的相位偏移相似,但用亚饱和脉冲处理时,观察到 -/- 偏移幅度增加了约 2 倍。在 -/- 视交叉上核 (SCN) 中观察到光诱导表达的相应升高。为了测试该表型是否基于视网膜水平的敏感性变化,测量了瞳孔收缩反应。在反应或视网膜组织学方面没有观察到差异,这表明表型发生在视网膜和视网膜下丘脑束之后。为了测试该表型是否由于时钟状态变量的幅度降低,评估了体内和 SCN 组织外植体中时钟基因和的表达。/- 小鼠的振幅、相位和周期长度正常。这些发现表明,ID2 通过控制时钟负性元件的光诱导,在 SCN 中央起搏器水平上参与光调节机制。

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