AI Article Synopsis

  • The purification of the origin recognition complex (ORC) from yeast has advanced studies on DNA replication, but traditional methods are complex and time-consuming due to genetic manipulations.
  • A new streamlined method using mammalian cells for co-transfection of modified plasmids simplifies the process, allowing for efficient overproduction of all six subunits of ORC without wild-type contamination.
  • This technique not only accelerates the acquisition of mutant ORCs but also has the potential to be applied to the purification of other protein complexes.

Article Abstract

Purification of the origin recognition complex (ORC) from wild-type budding yeast cells more than two decades ago opened up doors to analyze the initiation of eukaryotic chromosomal DNA replication biochemically. Although revised methods to purify ORC from overproducing cells were reported later, purification of mutant proteins using these systems still depends on time-consuming processes including genetic manipulation to construct and amplify mutant baculoviruses or yeast strains as well as several canonical protein fractionations. Here, we present a streamlined method to construct mutant overproducers, followed by purification of mutant ORCs. Use of mammalian cells co-transfected with conveniently mutagenized plasmids bearing a His tag excludes many of the construction and fractionation steps. Transfection is highly efficient. All the six subunits of ORC are overexpressed at a considerable level and isolated as a functional heterohexameric complex. Furthermore, use of mammalian cells prevents contamination of wild-type ORC from yeast cells. The method is applicable to wild-type and at least three mutant ORCs, and the resultant purified complexes show expected biochemical activities. The rapid acquisition of mutant ORCs using this system will boost systematic biochemical dissection of ORC and can be even applied to the purification of protein complexes other than ORC.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC4834435PMC
http://dx.doi.org/10.3389/fmicb.2016.00521DOI Listing

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