Supplementary Materials Supplemental Data supp_285_36_28229__index. of architectural elements and adversely supercoiled DNA, stimulates the melting of the adjacent AT-rich DNA-unwinding component (Thanks) (16,C20). Pursuing melting, DnaA collaborates with DnaC, the bacterial helicase loader, to deposit two hexamers from the DnaB helicase onto the foundation (14, 21,C24). DnaB subsequently nucleates replisome set up and unwinds the chromosome (3 processively, 25). The means where DnaA melts isn’t realized. The initiator itself can be a complicated, modular protein made up of four domains, including an N-terminal helicase-interaction site (23), a adjustable linker component, a central AAA+ fold that binds single-stranded (ss) DNA (26), and a C-terminal, helix-turn-helix DNA-binding site (DBD) that identifies duplex source sites (Fig. 1recognition and open up complex purchase PKI-587 formation can be unknown (10, 15, 16). The means by which the AAA+ element and the DBD coordinate their respective ssDNA- and double-stranded (ds)DNA-binding activities within the higher order DnaA complex similarly has not been resolved. Open in a separate window FIGURE 1. DnaA organization. and DnaA. Key motifs are purchase PKI-587 Mouse monoclonal to CK1 indicated. or and the AAA+ domains (77C310) colored either or by region. To address these issues, we conducted a series of mutagenesis, biochemical, and genetic studies of DnaA using available structures as a guide. Surprisingly, we found that crystallographically purchase PKI-587 observed interactions occurring in between the AAA+ domain of one DnaA protomer and the DBD of a partner subunit are necessary for both higher order initiator assembly and the binding of ssDNA. Moreover, this cross-talk is required for origin unwinding and global DnaA function DnaA (AaDnaA) constructs (residues 2C399, 76C399, 76C310, 290C399, and 1C80) were expressed as tobacco etch virus (TEV) protease-cleavable His6-maltose-binding protein (MBP) fusions. All AaDnaA proteins were purified as previously described (30), except for a few modifications described in supplemental Experimental Procedures. As a final purification step, untagged AaDnaA proteins were run over an S-200 size-exclusion column (GE Healthcare) in gel-filtration buffer (50 mm HEPES, pH 7.5, 500 mm KCl, 10% (v/v) glycerol, 5 mm MgCl2). Monomeric species were pooled, concentrated, and flash-frozen for storage at ?80 C. For mutagenesis studies, changes were introduced into His6-maltose-binding protein-AaDnaAAAA+/DBD (amino acids 76C399) using QuikChange mutagenesis (Stratagene). Expression and Purification of E. coli DnaA DnaA (EcDnaA) was expressed as a fusion with a tobacco etch virus protease-cleavable His6 tag. All His6-EcDnaA proteins were purified as previously described (40), except where noted in supplemental Experimental Procedures. As a final step, His6-EcDnaA proteins were passed over an S-200 sizing column and flash-frozen as per AaDnaA, except that 50 mm PIPES-KOH, pH 6.8, 10 mm magnesium acetate, 200 mm ammonium sulfate, 20% (v/v) sucrose, 0.1 mm EDTA, and 2 mm DTT was used as a gel-filtration buffer. Mutations were introduced into His6-EcDnaA using QuikChange mutagenesis. AaDnaA Cross-linking Assays Cross-linking was performed by incubating 50 g/ml of various AaDnaA proteins in 80 l of a reaction buffer (50 mm HEPES, pH 7.5, 10% (v/v) glycerol, 125 mm KCl, 5 mm MgCl2, 2 mm DTT) containing 2 mm nucleotide at 25 C for 5 min. Glutaraldehyde (Polysciences, Inc.) was then added to 1 mm final concentration using 8.8 l of a 10 mm stock. Reactions were incubated at 25 C for an additional 1 min before quenching with 8 l of 200 mm glycine, followed by the addition of 30 l of gel loading buffer (100.
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