RT Journal Article SR Electronic T1 Rapid isolation of functionally intact nuclei from the yeast Saccharomyces JF bioRxiv FD Cold Spring Harbor Laboratory SP 162388 DO 10.1101/162388 A1 Mario Niepel A1 Julia C. Farr A1 Michael P. Rout A1 Caterina Strambio-De-Castillia YR 2017 UL http://biorxiv.org/content/early/2017/07/12/162388.abstract AB Most available methods for nuclear isolation entail lengthy procedures that are difficult to master and generally emphasize yield and enrichment over nuclear preservation, thus limiting their utility for further studies. Here we demonstrate a novel and robust method to rapidly isolate well-preserved yeast nuclei. The method can be easily adapted to multiple preparation scales depending on experimental need and it can readily be performed on multiple samples by a single researcher in one day. We show that the nuclei fraction is strongly enriched and that the resulting nuclei are free from contaminating endoplasmatic reticulum and other cell debris. EM studies show that preservation of nuclear morphology is exquisite, making it possible to study peripheral nuclear pore components such as the cytoplasmic filaments and the basket, whose structure is generally difficult to maintain ex vivo. In addition, incubation of isolated nuclei with bulk transport substrates of different sizes and with import cargo indicates that the nuclear envelope is intact and nuclear pores retain their capacity to bind transport substrates. Our results suggest that this preparation procedure will greatly facilitate studies of the yeast nucleus which have been difficult to establish and to multiplex to date.