Becker David L, Webb Kevin F, Thrasivoulou Christopher, Lin Chih-Chi, Nadershahi Roxana, Tsakiri Niki, Cook Jeremy E
Department of Anatomy and Developmental Biology, University College London, Gower Street, London, UK.
J Physiol. 2007 Dec 15;585(Pt 3):711-9. doi: 10.1113/jphysiol.2007.138776. Epub 2007 Oct 11.
Neural progenitor cells in the developing retina extend processes that stretch from the basal vitread surface to the apical ventricular surface. During the cell cycle, the nucleus undergoes interkinetic nuclear migration (INM), moving in a vitread direction during G1, passing through S-phase at its peak and then, on entering G2, returning towards the ventricular surface where it enters M-phase and divides. We have previously shown that individual saltatory movements of the nucleus correlate with transient changes in cytosolic calcium concentration within these progenitor cells and that these events spread to neighbouring progenitors through connexin43 (Cx43) gap junction channels, thereby coordinating the migration of coupled clusters of cells. Disrupting coupling with pharmacological agents, Cx43-specific antisense oligodeoxynucleotides (asODNs) or dominant negative Cx43 (dnCx43) inhibits the sharing of calcium events, reducing the number that each cell experiences and significantly slowing INM. We have developed protocols for imaging migrating progenitor cells by confocal microscopy over relatively short periods, and by multiphoton microscopy over more extended periods that include complete cell cycles. We find that perturbing gap junctional communication not only slows the INM of progenitor cells but also apparently prevents them from changing direction at critical phases of the cell cycle. It also disrupts the migration of young neurons to their appropriate layers after terminal division and leads to their ectopic differentiation. The ability to perform extended time-lapse imaging over 3D volumes in living retina using multiphoton microscopy should now allow fundamental mechanisms governing development of the retinal neuroepithelium to be probed in detail.
发育中的视网膜中的神经祖细胞伸出的突起从玻璃体视网膜表面延伸至室管膜顶表面。在细胞周期中,细胞核经历核内运动(INM),在G1期向玻璃体视网膜方向移动,在S期达到峰值,然后进入G2期时返回室管膜表面,在那里进入M期并进行分裂。我们之前已经表明,细胞核的单个跳跃运动与这些祖细胞内细胞质钙浓度的瞬时变化相关,并且这些事件通过连接蛋白43(Cx43)间隙连接通道传播到相邻的祖细胞,从而协调耦合细胞簇的迁移。用药物制剂、Cx43特异性反义寡脱氧核苷酸(asODN)或显性负性Cx43(dnCx43)破坏耦合会抑制钙事件的共享,减少每个细胞经历的钙事件数量,并显著减缓核内运动。我们已经开发出了通过共聚焦显微镜在相对较短的时间内以及通过多光子显微镜在包括完整细胞周期的更长时间内对迁移的祖细胞进行成像的方案。我们发现,干扰间隙连接通讯不仅会减缓祖细胞的核内运动,而且显然会阻止它们在细胞周期的关键阶段改变方向。它还会破坏年轻神经元在终末分裂后向其适当层的迁移,并导致它们异位分化。现在,使用多光子显微镜在活体视网膜的三维体积上进行长时间延时成像的能力应该能够详细探究视网膜神经上皮发育的基本机制。