Method Article

Visualization of UV-induced Replication Intermediates in E. coli using Two-dimensional Agarose-gel Analysis

DOI:

10.3791/2220

December 21st, 2010

In This Article

Summary

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We present a procedure by which two-dimensional agarose-gel analysis can be used to identify the structure of replication intermediates that occur following UV irradiation.

Abstract

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Inaccurate replication in the presence of DNA damage is responsible for the majority of cellular rearrangements and mutagenesis observed in all cell types and is widely believed to be directly associated with the development of cancer in humans. DNA damage, such as that induced by UV irradiation, severely impairs the ability of replication to duplicate the genomic template accurately. A number of gene products have been identified that are required when replication encounters DNA lesions in the template. However, a remaining challenge has been to determine how these proteins process lesions during replication in vivo. Using Escherichia coli as a model system, we describe a procedure in which two-dimensional agarose-gel analysis can be used to identify the structural intermediates that arise on replicating plasmids in vivo following UV-induced DNA damage. This procedure has been used to demonstrate that replication forks blocked by UV-induced damage undergo a transient reversal that is stabilized by RecA and several gene products associated with the RecF pathway. The technique demonstrates that these replication intermediates are maintained until a time that correlates with the removal of the lesions by nucleotide excision repair and replication resumes.

Protocol

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1. Growth and UV Irradiation.

  1. 200μl of a fresh overnight culture containing the plasmid pBR322 grown in Davis medium1 supplemented with 0.4% glucose, 0.2% casamino acids, and 10 μg/ml thymine (DGCthy medium) and 100 μg/ml ampicillin is pelleted. The cell pellet is then resuspended in 200μl DGCthy medium lacking ampicillin and used to inoculate 20 ml of DGCthy medium.
  2. Cultures are grown without ampicillin selection in a shaking incubator at 37° C to an OD600 of 0.5 (~ 5 x 108 cells/ml). Growth without ampicillin avoids selection against abnormal or unproductive replication intermediates that may arise in some mu....

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Discussion

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Typical results obtained from wild type cells in the presence and absence of UV-induced damage are shown in Figure 1. In the absence of damage, ~1% of the total plasmid DNA can be found in the Y arc when cells are rapidly growing in exponential phase. Following irradiation, a transient increase in Y shaped molecules is observed as blocked replication forks accumulate at damaged sites. The X-shaped replication intermediates also transiently accumulate and persist until a time that correlates with when the lesions are rep.......

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Disclosures

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No conflicts of interest declared.

Acknowledgements

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Work in our lab is supported by CAREER award MCB0551798 from the National Science Foundation and AREA grant R15GM86839 from the NIGMS-NIH.

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Materials

List of materials used in this article
NameCompanyCatalog NumberComments
An example of the Southern analysis of the 2D gel probedGE HealthcareG15T8Yellow Lighting
15 μwatt germicidal lampSylvaniaF20T12/GOUV Lamp
Blak-Ray UV Intensity Meter 254nmDaiggerEF28195TUVC photometer
0.025 μm pore disksWhatman, GE HealthcareVSWP04700Floating dialysis disks
PvuIIFermentasER0632Restriction Endonuclease
Nick-translation kitRoche Group976776To make 32P-labeled probe
Blotting PaperWhatman, GE Healthcare3030-704For Southern transfer
Nylon membraneGE HealthcareRPN203SFor Southern transfer

References

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  1. Davis, B. D. The Isolation of Biochemically Deficient Mutants of Bacteria by Means of Penicillin. Proc Natl Acad Sci U S A. 35, 1-10 (1949).
  2. Courcelle, J., Donaldson, J. R., Chow, K. H., Courcelle, C. T. DNA Damage-Induced Replication Fork Regres....

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Tags

Two dimensional Gel ElectrophoresisDNA Replication IntermediatesUV induced DNA DamagePlasmid PBR322 AnalysisAgarose Gel AnalysisSouthern BlottingRestriction Enzyme DigestionAlkali Transfer SystemReplication Fork ReversalNucleotide Excision Repair

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