Marchenko Sergey M, Yarotskyy Victor V, Kovalenko Tatiana N, Kostyuk Platon G, Thomas Roger C
Bogomoletz Institute of Physiology, 4 Bogomoletz Street, Kiev, 01024, Ukraine.
J Physiol. 2005 Jun 15;565(Pt 3):897-910. doi: 10.1113/jphysiol.2004.081299. Epub 2005 Mar 17.
Increases in Ca(2+) concentration in the nucleus of neurones modulate gene transcription and may be involved in activity-dependent long-term plasticity, apoptosis, and neurotoxicity. Little is currently known about the regulation of Ca(2+) in the nuclei of neurones. Investigation of neuronal nuclei is hampered by the cellular heterogeneity of the brain where neurones comprise no more than 10% of the cells. The situation is further complicated by large differences in properties of different neurones. Here we report a method for isolating nuclei from identified central neurones. We employed this technique to study nuclei from rat cerebellar Purkinje and granule neurones. Patch-clamp recording from the nuclear membrane of Purkinje neurones revealed numerous large-conductance channels selective for monovalent cations. The nuclear membrane of Purkinje neurones also contained multiple InsP(3)- activated ion channels localized exclusively in the inner nuclear membrane with their receptor loci facing the nucleoplasm. In contrast, the nuclear membrane of granule neurones contained only a small number of mainly anion channels. Nuclear InsP(3) receptors (InsP(3)Rs) were activated by InsP(3) with EC(50) = 0.67 microm and a Hill coefficient of 2.5. Ca(2+) exhibited a biphasic effect on the receptors elevating its activity at low concentrations and inhibiting it at micromolar concentrations. InsP(3) in saturating concentrations did not prevent the inhibitory effect of Ca(2+), but strongly increased InsP(3)R activity at resting Ca(2+) concentrations. These data are the first evidence for the presence of intranuclear sources of Ca(2+) in neurones. Ca(2+) release from the nuclear envelope may amplify Ca(2+) transients penetrating the nucleus from the cytoplasm or generate Ca(2+) transients in the nucleus independently of the cytoplasm.
神经元细胞核中钙离子浓度的升高会调节基因转录,并可能参与依赖活动的长期可塑性、细胞凋亡和神经毒性。目前对神经元细胞核中钙离子的调节知之甚少。由于大脑细胞的异质性,其中神经元细胞占比不超过10%,因此对神经元细胞核的研究受到阻碍。不同神经元特性的巨大差异进一步使情况变得复杂。在此,我们报告一种从已鉴定的中枢神经元中分离细胞核的方法。我们采用该技术研究大鼠小脑浦肯野神经元和颗粒神经元的细胞核。对浦肯野神经元核膜进行膜片钳记录发现了许多对单价阳离子有选择性的大电导通道。浦肯野神经元的核膜还含有多个仅在内核膜中定位的肌醇三磷酸(InsP(3))激活离子通道,其受体位点面向核质。相比之下,颗粒神经元的核膜仅含有少量主要为阴离子通道。核内InsP(3)受体(InsP(3)Rs)被InsP(3)激活,其半数有效浓度(EC(50))为0.67微摩尔,希尔系数为2.5。钙离子对受体表现出双相作用,在低浓度时提高其活性,在微摩尔浓度时抑制其活性。饱和浓度的InsP(3)并不能阻止钙离子的抑制作用,但在静息钙离子浓度下能强烈增加InsP(3)R的活性。这些数据首次证明了神经元细胞核中存在钙离子的核内来源。从核膜释放的钙离子可能会放大从细胞质穿透细胞核的钙离子瞬变,或者独立于细胞质在细胞核中产生钙离子瞬变。