2000
DOI: 10.1126/science.287.5460.2023
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Start Sites of Bidirectional DNA Synthesis at the Human Lamin B2 Origin

Abstract: The initiation sites of bidirectional synthesis at the DNA replication origin located at the 3' end of the human lamin B2 gene were investigated. RNA-primed nascent DNA molecules were subjected to second-strand synthesis with appropriate primers, amplified by ligation-mediated polymerase chain reaction, and size fractionated. Evidence for precise start sites was obtained. Exploration of close to 1 kilobase, coupled to inhibition of Okazaki fragment synthesis, demonstrates that the leading strands initiate at p… Show more

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Cited by 172 publications
(186 citation statements)
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“…In yeast cells, one strategy to circumvent this problem is to compare RIPs in wild-type and DNA ligase I-deficient mutants 3 . Since this method is difficult to apply in mammalian cells, we and others used emetine, which inhibits new production of lagging strands without affecting leading strand synthesis 1,11 . Although concern was raised previously regarding drug treatments and the generation of potential artifactual results 2 , we did not observe any notable problemwhenwe determined DBF4 RIPs with cells maintained in the presence and absence of emetine 10 .…”
Section: Experimental Designmentioning
confidence: 99%
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“…In yeast cells, one strategy to circumvent this problem is to compare RIPs in wild-type and DNA ligase I-deficient mutants 3 . Since this method is difficult to apply in mammalian cells, we and others used emetine, which inhibits new production of lagging strands without affecting leading strand synthesis 1,11 . Although concern was raised previously regarding drug treatments and the generation of potential artifactual results 2 , we did not observe any notable problemwhenwe determined DBF4 RIPs with cells maintained in the presence and absence of emetine 10 .…”
Section: Experimental Designmentioning
confidence: 99%
“…Choice of DNA polymerases-Although Vent (exo − ) DNA polymerase has been the polymerase of choice for RIP mapping [1][2][3] , this enzyme was not ideal under our experimental conditions. The possible reason for this is that the activity of this polymerase may not be compatible with betaine.…”
Section: Experimental Designmentioning
confidence: 99%
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