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The function of the replication clamp loaders in the semi-conservative telomere replication and their relationship to telomerase- and recombination mechanisms of telomere addition remains ambiguous. We have investigated the variant clamp loader Ctf18 RFC (Replication Factor C). To understand the role of Ctf18 at the telomere, we first investigated genetic interactions after loss of Ctf18 and TLC1 (the yeast telomerase RNA). We find that the tlc1Δ ctf18Δ double mutant confers a rapid >1000-fold decrease in viability. The rate of loss was similar to the kinetics of cell death in rad52Δ tlc1Δ cells. However, the Ctf18 pathway is distinct from Rad52, required for the repair of DSBs, as demonstrated by the synthetic lethality of rad52▵ tlc1Δ ctf18Δ triple mutants. These data suggest that each mutant elicits non-redundant defects acting on the same substrate. Second, interactions of the yeast hyper-recombinational mutant, mre11A470T, with ctf18▵ confer a synergistic cold sensitivity. The phenotype of these double mutants ultimately results in telomere loss and the generation of recombinational survivors. We observed a similar synergism between single mutants that led to hypersensitivity to the DNA alkylating agent, methane methyl sulphonate (MMS), the replication fork inhibitor hydroxyurea (HU), and to a failure to separate telomeres of sister chromatids. Hence, ctf18Δ and mre11A470T act in different pathways on telomere substrates for multiple phenotypes. The mre11A470T cells also displayed a DNA damage response (DDR) at 15°C but not at 30°C while ctf18Δ mutants conferred a constitutive DDR activity. Both the 15°C DDR pattern and growth rate were reversible at 30°C and displayed telomerase activity in vivo. We hypothesize that Ctf18 confers protection against stalling and/or breaks at the replication fork in cells that either lack, or are compromised for, telomerase activity. This Ctf18-based function is likely to contribute another level to telomere size homeostasis.

Titel:	The Ctf18RFC clamp loader is essential for telomere stability in telomerase-negative and mre11 mutant alleles.
Autor/in / Beteiligte Person:	Gao, H ; Moss, DL ; Parke, C ; Tatum, D ; Lustig, AJ
Link:	Volltext (PDF)
Zeitschrift:	PloS one, Jg. 9 (2014-02-12), Heft 2, S. e88633
Veröffentlichung:	San Francisco, CA : Public Library of Science, 2014
Medientyp:	academicJournal
ISSN:	1932-6203 (electronic)
DOI:	10.1371/journal.pone.0088633
Schlagwort:	Alleles Cell Cycle Proteins metabolism Checkpoint Kinase 2 metabolism Chromatids chemistry DNA Repair Endodeoxyribonucleases metabolism Exodeoxyribonucleases metabolism Hydroxyurea chemistry Kinetics Methyl Methanesulfonate chemistry Phenotype Saccharomyces cerevisiae metabolism Temperature Endodeoxyribonucleases genetics Exodeoxyribonucleases genetics Mutation Replication Protein C metabolism Saccharomyces cerevisiae Proteins genetics Saccharomyces cerevisiae Proteins metabolism Telomerase metabolism Telomere ultrastructure
Sonstiges:	Nachgewiesen in: MEDLINE Sprachen: English Publication Type: Journal Article; Research Support, N.I.H., Extramural; Research Support, Non-U.S. Gov't Language: English [PLoS One] 2014 Feb 12; Vol. 9 (2), pp. e88633. <i>Date of Electronic Publication: </i>2014 Feb 12 (<i>Print Publication: </i>2014). MeSH Terms: Mutation* ; Endodeoxyribonucleases / genetics ; Exodeoxyribonucleases / genetics ; Replication Protein C / metabolism ; Saccharomyces cerevisiae Proteins / genetics ; Saccharomyces cerevisiae Proteins / metabolism ; Telomerase / metabolism ; Telomere / *ultrastructure ; Alleles ; Cell Cycle Proteins / metabolism ; Checkpoint Kinase 2 / metabolism ; Chromatids / chemistry ; DNA Repair ; Endodeoxyribonucleases / metabolism ; Exodeoxyribonucleases / metabolism ; Hydroxyurea / chemistry ; Kinetics ; Methyl Methanesulfonate / chemistry ; Phenotype ; Saccharomyces cerevisiae / metabolism ; Temperature References: J Biol Chem. 2013 Apr 19;288(16):11273-86. (PMID: 23443654) ; EMBO J. 2009 Apr 8;28(7):799-809. (PMID: 19214183) ; Proc Natl Acad Sci U S A. 2011 Nov 1;108(44):17927-32. (PMID: 22003126) ; PLoS Genet. 2011 Sep;7(9):e1002271. (PMID: 21931565) ; EMBO J. 2010 Oct 6;29(19):3370-80. (PMID: 20834227) ; Nat Struct Mol Biol. 2012 Feb 12;19(3):307-13. (PMID: 22343724) ; BMC Syst Biol. 2012 Jan 13;6:4. (PMID: 22244311) ; EMBO J. 2006 Apr 5;25(7):1505-14. (PMID: 16525505) ; Genes Dev. 1996 Jun 1;10(11):1310-26. (PMID: 8647430) ; Eukaryot Cell. 2010 Oct;9(10):1612-21. (PMID: 20709788) ; J Biol Chem. 2013 May 3;288(18):12840-51. (PMID: 23525106) ; Cancer Res. 2008 May 1;68(9):3115-23. (PMID: 18451136) ; Curr Biol. 2013 Jan 7;23(1):64-9. (PMID: 23219725) ; Curr Biol. 2006 May 9;16(9):902-6. (PMID: 16682351) ; Mol Cell Biol. 2002 Aug;22(16):5679-87. (PMID: 12138180) ; Proc Biol Sci. 2009 May 7;276(1662):1679-83. (PMID: 19324831) ; Cell. 1993 Apr 23;73(2):347-60. (PMID: 8477448) ; EMBO J. 1999 Jun 15;18(12):3509-19. (PMID: 10369690) ; Exp Cell Res. 2006 Aug 15;312(14):2654-9. (PMID: 16859682) ; Genetics. 1999 May;152(1):143-52. (PMID: 10224249) ; DNA Repair (Amst). 2005 Apr 4;4(4):409-17. (PMID: 15725622) ; Genetics. 2010 Jul;185(3):761-70. (PMID: 20421597) ; Mol Cell. 2007 Aug 17;27(4):550-61. (PMID: 17656141) ; J Biol Chem. 2004 Jan 2;279(1):223-30. (PMID: 14573610) ; Nucleic Acids Res. 2007;35(15):4989-5000. (PMID: 17636314) ; Eukaryot Cell. 2004 Apr;3(2):369-84. (PMID: 15075267) ; Mol Cell Biol. 2000 Mar;20(5):1659-68. (PMID: 10669743) ; PLoS One. 2010 Nov 30;5(11):e14142. (PMID: 21152442) ; EMBO J. 2009 Sep 16;28(18):2803-11. (PMID: 19680223) ; Science. 1994 Oct 21;266(5184):404-9. (PMID: 7545955) ; Nature. 1990 May 31;345(6274):456-8. (PMID: 2111466) ; Mol Cell. 2001 Jun;7(6):1255-66. (PMID: 11430828) ; Aging Cell. 2013 Aug;12(4):719-27. (PMID: 23672410) ; Mol Cell. 2003 Feb;11(2):303-13. (PMID: 12620220) ; PLoS Genet. 2011 Dec;7(12):e1002421. (PMID: 22194704) ; Mol Cell Biol. 2007 Sep;27(18):6532-45. (PMID: 17636027) ; Science. 1997 Feb 14;275(5302):986-90. (PMID: 9020083) ; DNA Repair (Amst). 2010 Dec 10;9(12):1283-91. (PMID: 21050828) ; RNA. 2006 Sep;12(9):1721-37. (PMID: 16894218) ; Nature. 2007 Aug 16;448(7155):820-3. (PMID: 17671506) ; PLoS Genet. 2009 May;5(5):e1000475. (PMID: 19424434) ; Mol Biol Cell. 2008 Feb;19(2):595-607. (PMID: 18045993) ; Mol Cell Biol. 2001 May;21(9):3144-58. (PMID: 11287619) ; Mol Cell Biol. 2001 Oct;21(19):6559-73. (PMID: 11533244) ; Cell Cycle. 2012 Apr 1;11(7):1309-15. (PMID: 22421147) ; Exp Cell Res. 2012 Jul 15;318(12):1456-60. (PMID: 22391099) ; Mol Cell Biol. 2014 Jan;34(1):57-70. (PMID: 24164896) ; Mol Cell. 2009 Jul 10;35(1):70-81. (PMID: 19595717) ; Proc Natl Acad Sci U S A. 1986 Mar;83(5):1398-402. (PMID: 3513174) ; Methods Mol Biol. 2009;521:169-90. (PMID: 19563106) ; Cell. 2011 Apr 1;145(1):54-66. (PMID: 21458667) ; Nat Struct Mol Biol. 2010 Dec;17(12):1438-45. (PMID: 21057524) ; Mol Cell. 2009 Feb 13;33(3):312-22. (PMID: 19217405) ; Prog Nucleic Acid Res Mol Biol. 2004;78:227-60. (PMID: 15210332) ; Nat Rev Mol Cell Biol. 2011 Feb;12(2):90-103. (PMID: 21252998) Substance Nomenclature: 0 (CTF18 protein, S cerevisiae) ; 0 (Cell Cycle Proteins) ; 0 (Saccharomyces cerevisiae Proteins) ; AT5C31J09G (Methyl Methanesulfonate) ; EC 2.7.1.11 (Checkpoint Kinase 2) ; EC 2.7.12.1 (RAD53 protein, S cerevisiae) ; EC 2.7.7.49 (Telomerase) ; EC 3.1.- (Endodeoxyribonucleases) ; EC 3.1.- (Exodeoxyribonucleases) ; EC 3.1.- (MRE11 protein, S cerevisiae) ; EC 3.6.4.- (Replication Protein C) ; X6Q56QN5QC (Hydroxyurea) Entry Date(s): Date Created: 20140218 Date Completed: 20150109 Latest Revision: 20231110 Update Code: 20231215 PubMed Central ID: PMC3923045

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The Ctf18RFC clamp loader is essential for telomere stability in telomerase-negative and mre11 mutant alleles.