By Palyl, Zucchi, Caglloti

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Mito. 03 M MC ~g pSP72 FIG. 2. Nucleic acid content of a typical minichromosome preparation. 8% (w/v) agarose gel containing ethidium bromide at 1/zg/ml. 5-kb TRPIARS1 plasmid with CUP1 inserted at the EcoRI site. 1-/zg supercoiled pSP72 vector (Promega), which is the same size as the minichromosomal DNA. The size marker (M) is a mixture of a BstEII digest of A DNA and an MspI digest of pBR322 (New England Biolabs, Beverly, MA). 48 ASSEMBLY OF NUCLEOSOMES, CHROMATIN, AND NUCLEI [3] 6. Transfer dialysate to microfuge tubes on ice: spin briefly in a refrigerated microfuge to remove any insoluble material.

The protocol presented here explains the preparation, from X. laevis oocytes, of an efficient extract that can assemble the large amounts of chromatin necessary for biochemical analysis. In addition, methods are described for the isolation of key nucleosome assembly components from the oocyte extract. Preparation of Xenopus Oocyte Extracts Toads, fed with fresh calf liver, are maintained in secured stainless-steel (or appropriate plastic) tanks in tap water (allowed to stand for 24 hr to permit dechlorination) at 20-24 °.

In this regard, the multigel apparatus required to measure the/x0 is relatively inexpensive, making it possible for virtually every chromatin laboratory to exploit the advantages inherent in the analysis of defined nucleosomal array and chromatin model systems if desired. Selective Enrichment of Saturated Nucleosomal Arrays Although with regular practice it is possible to achieve the optimal reconstitutes described earlier after the initial attempt, in general this is not an easy task to accomplish.

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