Large domain movements upon UvrD dimerization and helicase activation

Escherichia coli UvrD DNA helicase functions in several DNA repair processes. As a monomer, UvrD can translocate rapidly and processively along ssDNA; however, the monomer is a poor helicase. To unwind duplex DNA in vitro, UvrD needs to be activated either by self-assembly to form a dimer or by interaction with an accessory protein. However, the mechanism of activation is not understood. UvrD can exist in multiple conformations associated with the rotational conformational state of its 2B subdomain, and its helicase activity has been correlated with a closed 2B conformation. Using single-molecule total internal reflection fluorescence microscopy, we examined the rotational conformational states of the 2B subdomain of fluorescently labeled UvrD and their rates of interconversion. We find that the 2B subdomain of the UvrD monomer can rotate between an open and closed conformation as well as two highly populated intermediate states. The binding of a DNA substrate shifts the 2B conformation of a labeled UvrD monomer to a more open state that shows no helicase activity. The binding of a second unlabeled UvrD shifts the 2B conformation of the labeled UvrD to a more closed state resulting in activation of helicase activity. Binding of a monomer of the structurally similar Escherichia coli Rep helicase does not elicit this effect. This indicates that the helicase activity of a UvrD dimer is promoted via direct interactions between UvrD subunits that affect the rotational conformational state of its 2B subdomain.

Download Full-text

UvrD helicase activation by MutL involves rotation of its 2B subdomain

Proceedings of the National Academy of Sciences ◽

10.1073/pnas.1905513116 ◽

2019 ◽

Vol 116 (33) ◽

pp. 16320-16325 ◽

Cited By ~ 7

Author(s):

Yerdos A. Ordabayev ◽

Binh Nguyen ◽

Alexander G. Kozlov ◽

Haifeng Jia ◽

Timothy M. Lohman

Keyword(s):

Escherichia Coli ◽

Single Molecule ◽

Self Assembly ◽

Kinetic Studies ◽

Conformational State ◽

Helicase Activity ◽

Single Molecule Fret ◽

Open Conformation ◽

Dna Complex

Escherichia coli UvrD is a superfamily 1 helicase/translocase that functions in DNA repair, replication, and recombination. Although a UvrD monomer can translocate along single-stranded DNA, self-assembly or interaction with an accessory protein is needed to activate its helicase activity in vitro. Our previous studies have shown that an Escherichia coli MutL dimer can activate the UvrD monomer helicase in vitro, but the mechanism is not known. The UvrD 2B subdomain is regulatory and can exist in extreme rotational conformational states. By using single-molecule FRET approaches, we show that the 2B subdomain of a UvrD monomer bound to DNA exists in equilibrium between open and closed states, but predominantly in an open conformation. However, upon MutL binding to a UvrD monomer–DNA complex, a rotational conformational state is favored that is intermediate between the open and closed states. Parallel kinetic studies of MutL activation of the UvrD helicase and of MutL-dependent changes in the UvrD 2B subdomain show that the transition from an open to an intermediate 2B subdomain state is on the pathway to helicase activation. We further show that MutL is unable to activate the helicase activity of a chimeric UvrD containing the 2B subdomain of the structurally similar Rep helicase. Hence, MutL activation of the monomeric UvrD helicase is regulated specifically by its 2B subdomain.

Download Full-text

RuvA and RuvB proteins of Escherichia coli exhibit DNA helicase activity in vitro.

Proceedings of the National Academy of Sciences ◽

10.1073/pnas.90.4.1315 ◽

1993 ◽

Vol 90 (4) ◽

pp. 1315-1319 ◽

Cited By ~ 100

Author(s):

I. R. Tsaneva ◽

B. Muller ◽

S. C. West

Keyword(s):

Escherichia Coli ◽

Dna Helicase ◽

Helicase Activity

Download Full-text

N-terminal truncations on L1 proteins of human papillomaviruses promote their soluble expression in Escherichia coli and self-assembly in vitro

Emerging Microbes & Infections ◽

10.1038/s41426-018-0158-2 ◽

2018 ◽

Vol 7 (1) ◽

pp. 1-12 ◽

Cited By ~ 4

Author(s):

Minxi Wei ◽

Daning Wang ◽

Zhihai Li ◽

Shuo Song ◽

Xianglin Kong ◽

...

Keyword(s):

Escherichia Coli ◽

Self Assembly ◽

Human Papillomaviruses ◽

Soluble Expression ◽

Expression In Escherichia Coli

Download Full-text

Effects of Pathological Mutations on the Prion-Like Polymerisation of MyD88

10.1101/351726 ◽

2018 ◽

Author(s):

Ailís O’Carroll ◽

Brieuc Chauvin ◽

James Brown ◽

Ava Meagher ◽

Joanne Coyle ◽

...

Keyword(s):

Single Molecule ◽

Self Assembly ◽

Point Mutations ◽

Adaptor Protein ◽

Full Length ◽

Binary Response ◽

Death Domain ◽

Tir Domain ◽

The Impact

AbstractA novel concept has emerged whereby the higher-order self-assembly of proteins provides a simple and robust mechanism for signal amplification. This appears to be a universal signalling mechanism within the innate immune system, where the recognition of pathogens or danger-associated molecular patterns need to trigger a strong, binary response within cells. Previously, multiple structural studies have been limited to single domains, expressed and assembled at high protein concentrations. We therefore set out to develop new in vitro strategies to characterise the behaviour of full-length proteins at physiological levels. In this study we focus on the adaptor protein MyD88, which contains two domains with different self-assembly properties: a TIR domain that can polymerise similarly to the TIR domain of Mal, and a Death Domain that has been shown to oligomerise with helical symmetry in the Myddosome complex. To visualize the behaviour of full-length MyD88 without purification steps, we use single-molecule fluorescence coupled to eukaryotic cell-free protein expression. These experiments demonstrate that at low protein concentration, only full-length MyD88 forms prion-like polymers. We also demonstrate that the metastability of MyD88 polymerisation creates the perfect binary response required in innate signalling: the system is silenced at normal concentrations but upstream signalling creates a “seed” that triggers polymerisation and amplification of the response. These findings pushed us to re-interpret the role of polymerisation in MyD88-related diseases and we studied the impact of disease-associated point mutations L93P, R196C and L252P/L265P at the molecular level. We discovered that all mutations completely block the ability of MyD88 to polymerise. We also confirm that L252P, a gain-of-function mutation, allows the MyD88 mutant to form extremely stable oligomers, even when expressed at low nanomolar concentrations. Thus, our results are consistent with and greatly add to the findings on the Myddosomes digital ‘all-or-none’ responses and the behaviour of the oncogenic mutation of MyD88.

Download Full-text

Dynamic mechanisms of CRISPR interference by Escherichia coli CRISPR-Cas3

10.1101/2021.07.18.452824 ◽

2021 ◽

Author(s):

Kazuto Yoshimi ◽

Kohei TAKESHITA ◽

Noriyuki Kodera ◽

Satomi Shibumura ◽

Yuko Yamauchi ◽

...

Keyword(s):

Escherichia Coli ◽

High Speed ◽

Dna Helicase ◽

Type I ◽

Loop Formation ◽

Force Microscopy ◽

Atomic Force ◽

Target Strand ◽

Target Dna

Type I CRISPR-Cas3 uses an RNA-guided multi Cas-protein complex, Cascade, which detects and degrades foreign nucleic acids via the helicase-nuclease Cas3 protein. Despite many studies using cryoEM and smFRET, the precise mechanism of Cas3-mediated cleavage and degradation of target DNA remains elusive. Here we reconstitute the CRISPR-Cas3 system in vitro to show how the Escherichia coli Cas3 (EcoCas3) with EcoCascade exhibits collateral non-specific ssDNA cleavage and target specific DNA degradation. Partial binding of EcoCascade to target DNA with tolerated mismatches within the spacer sequence, but not the PAM, elicits collateral ssDNA cleavage activity of recruited EcoCas3. Conversely, stable binding with complete R-loop formation drives EcoCas3 to nick the non-target strand (NTS) in the bound DNA. Helicase-dependent unwinding then combines with trans ssDNA cleavage of the target strand and repetitive cis cleavage of the NTS to degrade the target dsDNA substrate. High-speed atomic force microscopy demonstrates that EcoCas3 bound to EcoCascade repeatedly reels and releases the target DNA, followed by target fragmentation. Together, these results provide a revised model for collateral ssDNA cleavage and target dsDNA degradation by CRISPR-Cas3, furthering understanding of type I CRISPR priming and interference and informing future genome editing tools.

Download Full-text

DNA Helicase Activity of PcrA Is Not Required for the Displacement of RecA Protein from DNA or Inhibition of RecA-Mediated Strand Exchange

Journal of Bacteriology ◽

10.1128/jb.00376-07 ◽

2007 ◽

Vol 189 (12) ◽

pp. 4502-4509 ◽

Cited By ~ 23

Author(s):

Syam P. Anand ◽

Haocheng Zheng ◽

Piero R. Bianco ◽

Sanford H. Leuba ◽

Saleem A. Khan

Keyword(s):

Dna Recombination ◽

Reca Protein ◽

Resonance Energy ◽

Dna Helicase ◽

Strand Exchange ◽

Single Pair ◽

Helicase Activity ◽

Dna Strand Exchange ◽

Dna Strand

ABSTRACT PcrA is a conserved DNA helicase present in all gram-positive bacteria. Bacteria lacking PcrA show high levels of recombination. Lethality induced by PcrA depletion can be overcome by suppressor mutations in the recombination genes recFOR. RecFOR proteins load RecA onto single-stranded DNA during recombination. Here we test whether an essential function of PcrA is to interfere with RecA-mediated DNA recombination in vitro. We demonstrate that PcrA can inhibit the RecA-mediated DNA strand exchange reaction in vitro. Furthermore, PcrA displaced RecA from RecA nucleoprotein filaments. Interestingly, helicase mutants of PcrA also displaced RecA from DNA and inhibited RecA-mediated DNA strand exchange. Employing a novel single-pair fluorescence resonance energy transfer-based assay, we demonstrate a lengthening of double-stranded DNA upon polymerization of RecA and show that PcrA and its helicase mutants can reverse this process. Our results show that the displacement of RecA from DNA by PcrA is not dependent on its translocase activity. Further, our results show that the helicase activity of PcrA, although not essential, might play a facilitatory role in the RecA displacement reaction.

Download Full-text

Characterization of the Helicase Activity and Substrate Specificity of Mycobacterium tuberculosis UvrD

Journal of Bacteriology ◽

10.1128/jb.01421-06 ◽

2006 ◽

Vol 189 (5) ◽

pp. 1542-1555 ◽

Cited By ~ 28

Author(s):

Elena Curti ◽

Stephen J. Smerdon ◽

Elaine O. Davis

Keyword(s):

Mycobacterium Tuberculosis ◽

Atpase Activity ◽

Amino Acid Identity ◽

Dna Helicase ◽

Helicase Activity ◽

Dna Oligonucleotides ◽

Promising Target ◽

Sites Of Action

ABSTRACT UvrD is a helicase that is widely conserved in gram-negative bacteria. A uvrD homologue was identified in Mycobacterium tuberculosis on the basis of the homology of its encoded protein with Escherichia coli UvrD, with which it shares 39% amino acid identity, distributed throughout the protein. The gene was cloned, and a histidine-tagged form of the protein was expressed and purified to homogeneity. The purified protein had in vitro ATPase activity that was dependent upon the presence of DNA. Oligonucleotides as short as four nucleotides were sufficient to promote the ATPase activity. The DNA helicase activity of the enzyme was only fueled by ATP and dATP. UvrD preferentially unwound 3′-single-stranded tailed duplex substrates over 5′-single-stranded ones, indicating that the protein had a duplex-unwinding activity with 3′-to-5′ polarity. A 3′ single-stranded DNA tail of 18 nucleotides was required for effective unwinding. By using a series of synthetic oligonucleotide substrates, we demonstrated that M. tuberculosis UvrD has an unwinding preference towards nicked DNA duplexes and stalled replication forks, representing the likely sites of action in vivo. The potential role of M. tuberculosis UvrD in maintenance of bacterial genomic integrity makes it a promising target for drug design against M. tuberculosis.

Download Full-text

Mechanistic insights into Lhr helicase function in DNA repair

Biochemical Journal ◽

10.1042/bcj20200379 ◽

2020 ◽

Vol 477 (16) ◽

pp. 2935-2947

Author(s):

Ryan J. Buckley ◽

Kevin Kramm ◽

Christopher D. O. Cooper ◽

Dina Grohmann ◽

Edward L. Bolt

Keyword(s):

Dna Repair ◽

Dna Replication ◽

Single Molecule ◽

Dna Helicase ◽

Holliday Junctions ◽

Single Molecule Fret ◽

Repair Enzymes ◽

Dna Strands

The DNA helicase Large helicase-related (Lhr) is present throughout archaea, including in the Asgard and Nanoarchaea, and has homologues in bacteria and eukaryotes. It is thought to function in DNA repair but in a context that is not known. Our data show that archaeal Lhr preferentially targets DNA replication fork structures. In a genetic assay, expression of archaeal Lhr gave a phenotype identical to the replication-coupled DNA repair enzymes Hel308 and RecQ. Purified archaeal Lhr preferentially unwound model forked DNA substrates compared with DNA duplexes, flaps and Holliday junctions, and unwound them with directionality. Single-molecule FRET measurements showed that binding of Lhr to a DNA fork causes ATP-independent distortion and base-pair melting at, or close to, the fork branchpoint. ATP-dependent directional translocation of Lhr resulted in fork DNA unwinding through the ‘parental’ DNA strands. Interaction of Lhr with replication forks in vivo and in vitro suggests that it contributes to DNA repair at stalled or broken DNA replication.

Download Full-text

Build Your Own Microscope: Step-By-Step Guide for Building a Prism-Based TIRF Microscope

Methods and Protocols ◽

10.3390/mps1040040 ◽

2018 ◽

Vol 1 (4) ◽

pp. 40 ◽

Cited By ~ 4

Author(s):

Dalton Gibbs ◽

Anisa Kaur ◽

Anoja Megalathan ◽

Kumar Sapkota ◽

Soma Dhakal

Keyword(s):

Single Molecule ◽

Total Internal Reflection ◽

Life Sciences ◽

Inverted Microscope ◽

Sophisticated Instrument ◽

High Level ◽

Single Molecule Analysis ◽

Molecule Dynamics ◽

Vast Range

Prism-based total internal reflection fluorescence (pTIRF) microscopy is one of the most widely used techniques for the single molecule analysis of a vast range of samples including biomolecules, nanostructures, and cells, to name a few. It allows for excitation of surface bound molecules/particles/quantum dots via evanescent field of a confined region of space, which is beneficial not only for single molecule detection but also for analysis of single molecule dynamics and for acquiring kinetics data. However, there is neither a commercial microscope available for purchase nor a detailed guide dedicated for building this microscope. Thus far, pTIRF microscopes are custom-built with the use of a commercially available inverted microscope, which requires high level of expertise in selecting and handling sophisticated instrument-parts. To directly address this technology gap, here we describe a step-by-step guide on how to build and characterize a pTIRF microscope for in vitro single-molecule imaging, nanostructure analysis and other life sciences research.

Download Full-text