Literature DB >> 27815898

Synchronization of Mammalian Cell Cultures by Serum Deprivation.

Thomas J Langan1,2,3,4, Kyla R Rodgers5, Richard C Chou6.   

Abstract

Mammalian cells are amenable to the study of regulatory mechanisms dictating cell cycle progression in vitro by shifting them into the same phase of the cycle. Procedures to arrest cultured cells in specific phases of the cell cycle may be termed in vitro synchronization. The procedure described here was developed for the study of primary astrocytes and a glioma cell line, but is broadly applicable to other mammalian cells. Its application allows astrocytes to re-enter the cell cycle from a state of quiescence (G0) under carefully defined experimental conditions to move together into subsequent phases such as the G1 and S phases. A number of methods have been established to synchronize mammalian cell cultures, which include counterflow centrifugal elutriation, mitotic shake off, chemically induced cell cycle arrest, and newer live cell methods, such as cell permeable dyes. Yet, there are intrinsic limitations associated with these methods. In the present protocol, we describe a simple, reliable, and reversible procedure to synchronize astrocyte and glioma cultures from newborn rat brain by serum deprivation. The procedure is similar, and generally applicable, to other mammalian cells. This protocol consists essentially of two parts: (1) proliferation of astrocytes under optimal conditions in vitro until reaching desired confluence; and (2) synchronization and G0 phase arrest of cultures by serum down-shift. This procedure has been utilized to examine cell cycle control in astroglioma cells and astrocytes from injured adult brain. It has also been employed in precursor cloning studies in developmental biology, suggesting wide applicability.

Entities:  

Keywords:  Astrocytes; Cell cycle; G0; Glioma; Serum deprivation; Synchronization

Mesh:

Substances:

Year:  2017        PMID: 27815898     DOI: 10.1007/978-1-4939-6603-5_6

Source DB:  PubMed          Journal:  Methods Mol Biol        ISSN: 1064-3745


  7 in total

1.  Preparation of Primary Acute Lymphoblastic Leukemia Cells in Different Cell Cycle Phases by Centrifugal Elutriation.

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2.  1α,25-Dihydroxyvitamin D3 (VD3) Shows a Neuroprotective Action Against Rotenone Toxicity on PC12 Cells: An In Vitro Model of Parkinson's Disease.

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Journal:  Neurochem Res       Date:  2022-09-06       Impact factor: 4.414

3.  Non-aggregated Aβ25-35 Upregulates Primary Astrocyte Proliferation In Vitro.

Authors:  Elise C Ohki; Thomas J Langan; Kyla R Rodgers; Richard C Chou
Journal:  Front Cell Neurosci       Date:  2017-09-26       Impact factor: 5.505

4.  Peptides Derived from (RRWQWRMKKLG)2-K-Ahx Induce Selective Cellular Death in Breast Cancer Cell Lines through Apoptotic Pathway.

Authors:  Diego Sebastián Insuasty-Cepeda; Andrea Carolina Barragán-Cárdenas; Alejandra Ochoa-Zarzosa; Joel E López-Meza; Ricardo Fierro-Medina; Javier Eduardo García-Castañeda; Zuly Jenny Rivera-Monroy
Journal:  Int J Mol Sci       Date:  2020-06-26       Impact factor: 5.923

5.  Priming mobilization of hair follicle stem cells triggers permanent loss of regeneration after alkylating chemotherapy.

Authors:  Jin Yong Kim; Jungyoon Ohn; Ji-Seon Yoon; Bo Mi Kang; Minji Park; Sookyung Kim; Woochan Lee; Sungjoo Hwang; Jong-Il Kim; Kyu Han Kim; Ohsang Kwon
Journal:  Nat Commun       Date:  2019-08-27       Impact factor: 14.919

6.  Innate Immune Functions of Astrocytes are Dependent Upon Tumor Necrosis Factor-Alpha.

Authors:  Kyla R Rodgers; Yufan Lin; Thomas J Langan; Yoichiro Iwakura; Richard C Chou
Journal:  Sci Rep       Date:  2020-04-27       Impact factor: 4.379

7.  Growth Factors Delivery System for Skin Regeneration: An Advanced Wound Dressing.

Authors:  Marta Nardini; Sara Perteghella; Luca Mastracci; Federica Grillo; Giorgio Marrubini; Elia Bari; Matteo Formica; Chiara Gentili; Ranieri Cancedda; Maria Luisa Torre; Maddalena Mastrogiacomo
Journal:  Pharmaceutics       Date:  2020-02-03       Impact factor: 6.321

  7 in total

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