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      A high ratio of G1 to G0 phase cells and an accumulation of G1 phase cells before S phase progression after injurious stimuli in the proximal tubule

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          Abstract

          Proximal tubule (PT) cells can proliferate explosively after injurious stimuli. To investigate this proliferative capacity, we examined cell cycle status and the expression of cyclin‐dependent kinase inhibitor p27, a G1 phase mediator, in PT cells after a proliferative or injurious stimulus. Rats were treated with lead acetate (proliferative stimulus) or uranyl acetate (UA; injurious stimulus). Isolated tubular cells were separated into PT and distal tubule (DT) cells by density‐gradient centrifugation. Cell cycle status was analyzed with flow cytometry by using the Hoechst 33342/pyronin Y method. Most PT and DT cells from control rats were in G0/G1 phase, with a higher percentage of PT cells than DT cells in G1 phase. Lead acetate and UA administration promoted the G0‐G1 transition and the accumulation of G1 phase cells before S phase progression. In PT cells from rats treated with lead acetate or a subnephrotoxic dose of UA, p27 levels increased or did not change, possibly reflecting G1 arrest. In contrast, p27 became undetectable before the appearance of apoptotic cells in rats treated with a nephrotoxic dose of UA. The decrease in p27 might facilitate rapid cell cycling. The decreased number of p27‐positive cells was associated with PT cell proliferation in renal tissues after a proliferative or injurious stimulus. The findings suggest that a high ratio of G1 to G0 phase cells and a rapid accumulation of G1 phase cells before S phase progression in the PT is a biological strategy for safe, timely, and explosive cell proliferation in response to injurious stimuli.

          Abstract

          Our results suggest that the ratio of G1 to G0 phase cells in the proximal tubule is higher than that in the distal tubule under physiological conditions. They also indicate that G1 phase cells accumulate rapidly before S phase progression in response to a proliferative or injurious stimulus. Our findings implicate p27 in G1 phase cell accumulation and S phase progression in the proximal tubule.

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          Inhibition of eukaryotic DNA replication by geminin binding to Cdt1.

          J A Wohlschlegel, B T Dwyer, S. K. Dhar (2000)
          In all eukaryotic organisms, inappropriate firing of replication origins during the G2 phase of the cell cycle is suppressed by cyclin-dependent kinases. Multicellular eukaryotes contain a second putative inhibitor of re-replication called geminin. Geminin is believed to block binding of the mini-chromosome maintenance (MCM) complex to origins of replication, but the mechanism of this inhibition is unclear. Here we show that geminin interacts tightly with Cdt1, a recently identified replication initiation factor necessary for MCM loading. The inhibition of DNA replication by geminin that is observed in cell-free DNA replication extracts is reversed by the addition of excess Cdt1. In the normal cell cycle, Cdt1 is present only in G1 and S, whereas geminin is present in S and G2 phases of the cell cycle. Together, these results suggest that geminin inhibits inappropriate origin firing by targeting Cdt1.
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            Isolation of quiescent and nonquiescent cells from yeast stationary-phase cultures

            Chris Allen, Sabrina Büttner, Anthony Aragon (2006)
            Quiescence is the most common and, arguably, most poorly understood cell cycle state. This is in part because pure populations of quiescent cells are typically difficult to isolate. We report the isolation and characterization of quiescent and nonquiescent cells from stationary-phase (SP) yeast cultures by density-gradient centrifugation. Quiescent cells are dense, unbudded daughter cells formed after glucose exhaustion. They synchronously reenter the mitotic cell cycle, suggesting that they are in a G0 state. Nonquiescent cells are less dense, heterogeneous, and composed of replicatively older, asynchronous cells that rapidly lose the ability to reproduce. Microscopic and flow cytometric analysis revealed that nonquiescent cells accumulate more reactive oxygen species than quiescent cells, and over 21 d, about half exhibit signs of apoptosis and necrosis. The ability to isolate both quiescent and nonquiescent yeast cells from SP cultures provides a novel, tractable experimental system for studies of quiescence, chronological and replicative aging, apoptosis, and the cell cycle.
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              p45SKP2 promotes p27Kip1 degradation and induces S phase in quiescent cells.

              H Sutterlüty, E Chatelain, A. Marti (1999)
              The F-box protein p45SKP2 is the substrate-targeting subunit of the ubiquitin-protein ligase SCFSKP2 and is frequently overexpressed in transformed cells. Here we report that expression of p45SKP2 in untransformed fibroblasts activates DNA synthesis in cells that would otherwise growth-arrest. Expression of p45SKP2 in quiescent fibroblasts promotes p27Kip1 degradation, allows the generation of cyclin-A-dependent kinase activity and induces S phase. Coexpression of a degradation-resistant p27Kip1 mutant suppresses p45SKP2-induced cyclin-A-kinase activation and S-phase entry. We propose that p45SKP2 is important in the progression from quiescence to S phase and that the ability of p45SKP2 to promote p27Kip1 degradation is a key aspect of its S-phase-inducing function. In transformed cells, p45SKP2 may contribute to deregulated initiation of DNA replication by interfering with p27Kip1 function.
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                Author and article information

                Journal
                Journal ID (nlm-ta): Physiol Rep
                Journal ID (iso-abbrev): Physiol Rep
                Journal ID (hwp): physreports
                Journal ID (publisher-id): phy2
                Title: Physiological Reports
                Publisher: Wiley Periodicals, Inc.
                ISSN (Electronic): 2051-817X
                Publication date Collection: October 2014
                Publication date (Electronic): 7 October 2014
                Volume: 2
                Issue: 10
                Electronic Location Identifier: e12173
                Affiliations
                [1 ]Internal Medicine I, Division of Nephrology, Hamamatsu University School of Medicine, Hamamatsu, Japan
                [2 ]Department of Internal Medicine, Teikyo University School of Medicine, Tokyo, Japan
                [3 ]Blood Purification Unit, Hamamatsu University School of Medicine, Hamamatsu, Japan
                Author notes
                CorrespondenceYoshihide Fujigaki, Department of Medicine, Teikyo University School of Medicine, 2‐11‐1 kaga, Itabashi‐ku, Tokyo 173‐8605, Japan. Tel: +81‐3‐3964‐1211 Fax: +81‐3‐3964‐8942 E‐mail: fujigaki@ 123456med.teikyo-u.ac.jp
                Article
                Publisher ID: phy212173
                DOI: 10.14814/phy2.12173
                PMC ID: 4254098
                PubMed ID: 25293601
                SO-VID: 02751937-eef6-4eff-a29f-267e4debbd07
                Copyright © © 2014 The Authors. Physiological Reports published by Wiley Periodicals, Inc. on behalf of the American Physiological Society and The Physiological Society.
                License:

                This is an open access article under the terms of the Creative Commons Attribution License, which permits use, distribution and reproduction in any medium, provided the original work is properly cited.

                History
                Date received : 08 September 2014
                Date revision received : 09 September 2014
                Date accepted : 10 September 2014
                Categories
                Subject: Original Research

                Keywords: cell cycle,g0‐g1 transition,g1 arrest,proximal tubule
                Data availability:
                Keywords: cell cycle, g0‐g1 transition, g1 arrest, proximal tubule

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