Published: Vol 8, Iss 17, Sep 5, 2018 DOI: 10.21769/BioProtoc.2994 Views: 32393
Reviewed by: Jia LiZinan ZhouShweta Garg
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Abstract
Cell synchronization is widely used in studying mechanisms involves in regulation of cell cycle progression. Through synchronization, cells at distinct cell cycle stage could be obtained. Thymidine is a DNA synthesis inhibitor that can arrest cell at G1/S boundary, prior to DNA replication. Here, we present the protocol to synchronize cells at G1/S boundary by using double thymidine block. After release into normal medium, cell population at distinct cell cycle phase could be collected at different time points.
Keywords: Cell synchronizationBackground
Cell cycle and cell division lie at the heart of cell biology. To build multicellular organism, cell duplication is necessary to generate specialized cells, which can execute particular function. The normal cell cycle is composed of interphase (G1, S and G2 phase) and mitotic (M) phase (Rodríguez-Ubreva et al., 2010; Léger et al., 2016). During interphase, the genetic materials are duplicated and make everything ready for mitosis. Whereas, during mitotic phase, the duplicated chromosomes are segregated and distributed into daughter cells (Sakaue-Sawano et al., 2008).
To precisely preserve genetic information, cell cycle progression must be tightly regulated. Cyclin/CDK complexes control the cell cycle progression through rapidly promoting activities at their respective stages, and are quickly inactivated when their stages are completed (Graña and Reddy, 1995).
Cell synchronization is particularly useful for investigating a cell-cycle regulated event. Using different methods, cells could be synchronized at different cell cycle stage. Treatment of nocodazole, which is an inhibitor of microtubule formation, could synchronize cells at G2/M phase (Ho et al., 2001), while, hydroxyurea, a dNTP synthesis inhibitor, synchronize cells at early S phase (Koç et al., 2004). As an Inhibitor of DNA synthesis (Schvartzman et al., 1984), thymidine can arrest cell at G1/S boundary. Here, we describe a detail method to synchronize cells at G1/S boundary by thymidine (Chen et al., 2018).
Materials and Reagents
Equipment
Procedure
Data analysis
Cell cycle was analyzed by flow cytometry with Flowjo software (Figure 1A). Cyclin A, Cyclin B and β-actin were detected by Western blotting (Figure 1B). Data are the representative of three independent experiments.
Notes
Recipes
Acknowledgments
This work was supported by NIH/NCI grants R01CA193828, R01CA136534 and R01CA200905 (to X. Deng), by the Winship Research Pathology and Integrated Cellular Imaging shared resource and the Emory Comprehensive Glycomics Core (ECGC) supported by the Winship Cancer Institute of Emory University (P30CAJ 38292), by the Winship Fashion a Cure Research Scholar Award (to X. Deng), a philanthropic award provided by the Winship, and by the Winship Endowment Fund (to XD). This protocol was adapted from our previous work (Chen et al., 2018).
Competing interests
The authors have declared that no conflict of interest exists.
References
Article Information
Copyright
© 2018 The Authors; exclusive licensee Bio-protocol LLC.
How to cite
Chen, G. and Deng, X. (2018). Cell Synchronization by Double Thymidine Block. Bio-protocol 8(17): e2994. DOI: 10.21769/BioProtoc.2994.
Category
Cancer Biology > Cell cycle checkpoints > Cell biology assays
Cell Biology > Cell signaling > Intracellular Signaling
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