Unusual regioversatility of acetyltransferase Eis, a cause of drug resistance in XDR-TB
The emergence of multidrug-resistant and extensively drug-resistant (XDR) tuberculosis (TB) is a serious global threat. Aminoglycoside antibiotics are used as a last resort to treat XDR-TB. Resistance to the aminoglycoside kanamycin is a hallmark of XDR-TB. Here, we reveal the function and structure of the mycobacterial protein Eis responsible for resistance to kanamycin in a significant fraction of kanamycin-resistant Mycobacterium tuberculosis clinical isolates. We demonstrate that Eis has an unprecedented ability to acetylate multiple amines of many aminoglycosides. Structural and mutagenesis studies of Eis indicate that its acetylation mechanism is enabled by a complex tripartite fold that includes two general control non-derepressible 5 (GCN5)-related N -acetyltransferase regions. An intricate negatively charged substrate-binding pocket of Eis is a potential target of new antitubercular drugs expected to overcome aminoglycoside resistance.
Site-specific DNA recombination is important for basic cellular functions including viral integration, control of gene expression, production of genetic diversity and segregation of newly replicated chromosomes, and is used by bacteriophage λ to integrate or excise its genome into and out of the host chromosome. λ recombination is carried out by the bacteriophage-encoded integrase protein (λ -int) together with accessory DNA sites and associated bending proteins that allow regulation in response to cell physiology. Here we report the crystal structures of λ -int in higher-order complexes with substrates and regulatory DNAs representing different intermediates along the reaction pathway. The structures show how the simultaneous binding of two separate domains of λ -int to DNA facilitates synapsis and can specify the order of DNA strand cleavage and exchange. An intertwined layer of amino-terminal domains bound to accessory (arm) DNAs shapes the recombination complex in a way that suggests how arm binding shifts the reaction equilibrium in favour of recombinant products.λ -int catalyses an ordered, pair-wise exchange of four DNA strands between two different pairs of recombination substrates 1,2 . During integration, λ -int aligns the bacteriophage attachment site attP with the bacterial attachment site attB and recombines these sequences to generate the recombination joints attL and attR flanking the integrated prophage (Fig. 1a, b). During the transition to lytic growth, the bacteriophage DNA is excised to regenerate attP and attB. In both reactions, the analogous pair of DNA strands ('top' strands) is exchanged first 3,4 to form a branched, four-way DNA intermediate known as a Holliday junction. Subsequent exchange of 'bottom' strands resolves the Holliday junction into linear recombinant products 2 . Although integration and excision might appear to be reciprocal reactions ( Fig. 1), they involve different substrates and are effectively irreversible 5 . The recombination machinery is configured differently during integration or excision by two different overlapping subsets of accessory factors and binding sites that bend the DNA arms flanking the core sites of strand exchange 2,6 . DNA bending is a prerequisite for the simultaneous interactions with arm and core sites 6-9 that deliver λ -int to lower-affinity core sites 10 . Arm-binding interactions allosterically enhance the fidelity of DNA strand exchange 11 and bias the outcome of Holliday junction resolution in favour of the recombined products 12 .Correspondence and requests for materials should be addressed to T.E. (tome@hms.harvard.edu).. * These authors contributed equally to this work.Supplementary Information is linked to the online version of the paper at www.nature.com/nature. These structures suggest that only a small shift in subunit packing is sufficient to redirect DNA cleavage and exchange activities from one pair of strands to the other, in order to resolve the Holliday junction into products 13,14 . However, the molecular mechanism o...
Purification and Characterization of Human NTH1, a Homolog ofEscherichia coli Endonuclease III
The human endonuclease III (hNTH1), a homolog of the Escherichia coli enzyme (Nth), is a DNA glycosylase with abasic (apurinic/apyrimidinic (AP)) lyase activity and specifically cleaves oxidatively damaged pyrimidines in DNA. Its cDNA was cloned, and the full-length enzyme (304 amino acid residues) was expressed as a glutathione S-transferase fusion polypeptide in E. coli. Purified wild-type protein with two additional amino acid residues and a truncated protein with deletion of 22 residues at the NH 2 terminus were equally active and had absorbance maxima at 280 and 410 nm, the latter due to the presence of a [4Fe-4S]cluster, as in E. coli Nth. The enzyme cleaved thymine glycol-containing form I plasmid DNA and a dihydrouracil (DHU)-containing oligonucleotide duplex. The protein had a molar extinction coefficient of 5.0 ؋ 10 4 and a pI of 10. With the DHU-containing oligonucleotide duplex as substrate, the K m was 47 nM, and k cat was ϳ0.6/min, independent of whether DHU paired with G or A. The enzyme carries out -elimination and forms a Schiff base between the active site residue and the deoxyribose generated after base removal. The prediction of Lys-212 being the active site was confirmed by sequence analysis of the peptideoligonucleotide adduct. Furthermore, replacing Lys-212 with Gln inactivated the enzyme. However, replacement with Arg-212 yielded an active enzyme with about 85-fold lower catalytic specificity than the wild-type protein. DNase I footprinting with hNTH1 showed protection of 10 nucleotides centered around the base lesion in the damaged strand and a stretch of 15 nucleotides (with the G opposite the lesion at the 5-boundary) in the complementary strand. Immunological studies showed that HeLa cells contain a single hNTH species of the predicted size, localized in both the nucleus and the cytoplasm.Reactive oxygen species are generated as by-products of oxidative phosphorylation or by ionizing radiation and induce extensive base damage that is mainly repaired via the base excision repair (BER) 1 pathway. This repair is initiated by removal of the damaged base, catalyzed by a DNA glycosylase (1-3). There are two classes of DNA glycosylases with distinct substrate specificities: the monofunctional simple glycosylase and the glycosylase with associated AP lyase activity. All oxidized base lesions are removed from DNA by DNA glycosylase/AP lyases, which not only catalyze removal of the base lesion but also cause strand cleavage via -elimination. The Escherichia coli endonuclease III (Nth) recognizes a wide range of oxidized pyrimidine derivatives, including ring-saturated and ring-fragmented derivatives such as thymine glycol (Tg), 5-hydroxycytosine, 5,6-dihydrouracil (DHU), and urea (1, 3-6). This enzyme has been well conserved from E. coli to the humans (7,8). On the other hand, oxidized purine lesions are also repaired by DNA glycosylase/AP lyases, i.e. Mut M (Fpg) of E. coli or OGG of eukaryotes (yeast and mammals), which do not share extensive sequence similarity. Furthermore, unlike these e...
No vaccine exists against group A Streptococcus (GAS), a leading cause of worldwide morbidity and mortality. A severe hurdle is the hypervariability of its major antigen, the M protein, with >200 different M types known. Neutralizing antibodies typically recognize M protein hypervariable regions (HVRs) and confer narrow protection. In stark contrast, human C4b-binding protein (C4BP), which is recruited to the GAS surface to block phagocytic killing, interacts with a remarkably large number of M protein HVRs (apparently ~90%). Such broad recognition is rare, and we discovered a unique mechanism for this through structure determination of four sequence-diverse M proteins in complex with C4BP. The structures revealed a uniform and tolerant ‘reading head’ in C4BP, which detected conserved sequence patterns hidden within hypervariability. Our results open up possibilities for rational therapies targeting the M-C4BP interaction, and also inform a path towards vaccine design.
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