Attempts to develop an enzyme converting DHIV to KIV

Abstract Dihydroxy-acid dehydratase (DHAD) catalyzes the dehydration of R-2,3-dihydroxyisovalerate (DHIV) to 2-ketoisovalerate (KIV) using an Fe-S cluster as a cofactor, which is sensitive to oxidation and expensive to synthesize. In contrast, sugar acid dehydratases catalyze the same chemical reactions using a magnesium ion. Here, we attempted to substitute the high-cost DHAD with a cost-efficient engineered sugar acid dehydratase using computational protein design (CPD). First, we tried without success to modify the binding pocket of a sugar acid dehydratase to accommodate the smaller, more hydrophobic DHIV. Then, we used a chemically activated substrate analog to react with sugar acid dehydratases or other enolase superfamily enzymes. Mandelate racemase from Pseudomonas putida (PpManR) and the putative sugar acid dehydratase from Salmonella typhimurium (StPutD) showed beta-elimination activity towards chlorolactate (CLD). CPD combined with medium-throughput selection improved the PpManR kcat/KM for CLD by four-fold. However, these enzyme variants did not show dehydration activity towards DHIV. Lastly, assuming phosphorylation could also be a good activation mechanism, we found that mevalonate-3-kinase (M3K) from Picrophilus torridus (PtM3K) exhibited adenosine triphosphate (ATP) hydrolysis activity when mixed with DHIV, indicating phosphorylation activity towards DHIV. Engineering PpManR or StPutD to accept 3-phospho-DHIV as a substrate was performed, but no variants with the desired activity were obtained.

Download Full-text

Engineering a light-controlled F1ATPase using structure-based protein design

PeerJ ◽

10.7717/peerj.2286 ◽

2016 ◽

Vol 4 ◽

pp. e2286 ◽

Cited By ~ 4

Author(s):

Daniel Hoersch

Keyword(s):

Protein Design ◽

Active Site ◽

Atp Hydrolysis ◽

Site Specific ◽

Dynamic Constraint ◽

End Distance ◽

A Site ◽

Hydrolysis Activity

The F1sub-complex of ATP synthase is a biological nanomotor that converts the free energy of ATP hydrolysis into mechanical work with an astonishing efficiency of up to 100% (Kinosita et al., 2000). To probe the principal mechanics of the machine, I re-engineered the active site ofE.coliF1ATPase with a structure-based protein design approach: by incorporation of a site-specific, photoswitchable crosslinker, whose end-to-end distance can be modulated by illumination with light of two different wavelengths, a dynamic constraint was imposed on the inter-atomic distances of the α and β subunits. Crosslinking reduced the ATP hydrolysis activity of four designs tested in vitro and in one case created a synthetic ATPase whose activity can be reversibly modulated by subsequent illumination with near UV and blue light. The work is a first step into the direction of the long-term goal to design nanoscaled machines based on biological parts that can be precisely controlled by light.

Download Full-text

Analysis of the crystal structure of an active MCM hexamer

eLife ◽

10.7554/elife.03433 ◽

2014 ◽

Vol 3 ◽

Cited By ~ 42

Author(s):

Justin M Miller ◽

Buenafe T Arachea ◽

Leslie B Epling ◽

Eric J Enemark

Keyword(s):

Crystal Structure ◽

Atp Hydrolysis ◽

Pyrococcus Furiosus ◽

Binding Pocket ◽

Activation Mechanism ◽

Binding Motif ◽

Atpase Domain ◽

Ssdna Binding ◽

Allosteric Communication ◽

Mcm Helicase

In a previous Research article (<xref ref-type="bibr" rid="bib25">Froelich et al., 2014</xref>), we suggested an MCM helicase activation mechanism, but were limited in discussing the ATPase domain because it was absent from the crystal structure. Here we present the crystal structure of a nearly full-length MCM hexamer that is helicase-active and thus has all features essential for unwinding DNA. The structure is a chimera of Sulfolobus solfataricus N-terminal domain and Pyrococcus furiosus ATPase domain. We discuss three major findings: 1) a novel conformation for the A-subdomain that could play a role in MCM regulation; 2) interaction of a universally conserved glutamine in the N-terminal Allosteric Communication Loop with the AAA+ domain helix-2-insert (h2i); and 3) a recessed binding pocket for the MCM ssDNA-binding motif influenced by the h2i. We suggest that during helicase activation, the h2i clamps down on the leading strand to facilitate strand retention and regulate ATP hydrolysis.

Download Full-text

Motif V regulates energy transduction between the flavivirus NS3 ATPase and RNA-binding cleft

Journal of Biological Chemistry ◽

10.1074/jbc.ra119.011922 ◽

2019 ◽

Vol 295 (6) ◽

pp. 1551-1564 ◽

Cited By ~ 5

Author(s):

Kelly E. Du Pont ◽

Russell B. Davidson ◽

Martin McCullagh ◽

Brian J. Geiss

Keyword(s):

Molecular Dynamics ◽

Structural Changes ◽

Rna Binding ◽

Atp Hydrolysis ◽

Nonstructural Protein ◽

Binding Pocket ◽

Energy Transduction ◽

Helicase Domain ◽

Genome Replication ◽

Turnover Rates

The unwinding of dsRNA intermediates is critical for the replication of flavivirus RNA genomes. This activity is provided by the C-terminal helicase domain of viral nonstructural protein 3 (NS3). As a member of the superfamily 2 (SF2) helicases, NS3 requires the binding and hydrolysis of ATP/NTP to translocate along and unwind double-stranded nucleic acids. However, the mechanism of energy transduction between the ATP- and RNA-binding pockets is not well-understood. Previous molecular dynamics simulations conducted by our group have identified Motif V as a potential “communication hub” for this energy transduction pathway. To investigate the role of Motif V in this process, here we combined molecular dynamics, biochemistry, and virology approaches. We tested Motif V mutations in both the replicon and recombinant protein systems to investigate viral genome replication, RNA-binding affinity, ATP hydrolysis activity, and helicase-mediated unwinding activity. We found that the T407A and S411A substitutions in NS3 reduce viral replication and increase the helicase-unwinding turnover rates by 1.7- and 3.5-fold, respectively, suggesting that flaviviruses may use suboptimal NS3 helicase activity for optimal genome replication. Additionally, we used simulations of each mutant to probe structural changes within NS3 caused by each mutation. These simulations indicate that Motif V controls communication between the ATP-binding pocket and the helical gate. These results help define the linkage between ATP hydrolysis and helicase activities within NS3 and provide insight into the biophysical mechanisms for ATPase-driven NS3 helicase function.

Download Full-text

Mitochondrial Lon protease is a gatekeeper for proteins newly imported into the matrix

Communications Biology ◽

10.1038/s42003-021-02498-z ◽

2021 ◽

Vol 4 (1) ◽

Author(s):

Yuichi Matsushima ◽

Kazuya Takahashi ◽

Song Yue ◽

Yuki Fujiyoshi ◽

Hideaki Yoshioka ◽

...

Keyword(s):

Protease Activity ◽

Matrix Protein ◽

Protein Import ◽

Atp Hydrolysis ◽

Lon Protease ◽

Mitochondrial Matrix ◽

The Matrix ◽

Specific Proteins ◽

Aggregation Activity ◽

Hydrolysis Activity

AbstractHuman ATP-dependent Lon protease (LONP1) forms homohexameric, ring-shaped complexes. Depletion of LONP1 causes aggregation of a broad range of proteins in the mitochondrial matrix and decreases the levels of their soluble forms. The ATP hydrolysis activity, but not protease activity, of LONP1 is critical for its chaperone-like anti-aggregation activity. LONP1 forms a complex with the import machinery and an incoming protein, and protein aggregation is linked with matrix protein import. LONP1 also contributes to the degradation of imported, aberrant, unprocessed proteins using its protease activity. Taken together, our results show that LONP1 functions as a gatekeeper for specific proteins imported into the mitochondrial matrix.

Download Full-text

Purification and Biochemical Characterization of the F1Fo-ATP Synthase from Thermoalkaliphilic Bacillus sp. Strain TA2.A1

Journal of Bacteriology ◽

10.1128/jb.185.15.4442-4449.2003 ◽

2003 ◽

Vol 185 (15) ◽

pp. 4442-4449 ◽

Cited By ~ 45

Author(s):

Gregory M. Cook ◽

Stefanie Keis ◽

Hugh W. Morgan ◽

Christoph von Ballmoos ◽

Ulrich Matthey ◽

...

Keyword(s):

Atp Synthase ◽

Biochemical Characterization ◽

Atp Hydrolysis ◽

Sodium Dodecyl ◽

Electrical Potential ◽

Atp Synthesis ◽

Intrinsic Property ◽

Protein Sequencing ◽

Hydrolysis Activity

ABSTRACT We describe here purification and biochemical characterization of the F1Fo-ATP synthase from the thermoalkaliphilic organism Bacillus sp. strain TA2.A1. The purified enzyme produced the typical subunit pattern of an F1Fo-ATP synthase on a sodium dodecyl sulfate-polyacrylamide gel, with F1 subunits α, β, γ, δ, and ε and Fo subunits a, b, and c. The subunits were identified by N-terminal protein sequencing and mass spectroscopy. A notable feature of the ATP synthase from strain TA2.A1 was its specific blockage in ATP hydrolysis activity. ATPase activity was unmasked by using the detergent lauryldimethylamine oxide (LDAO), which activated ATP hydrolysis >15-fold. This activation was the same for either the F1Fo holoenzyme or the isolated F1 moiety, and therefore latent ATP hydrolysis activity is an intrinsic property of F1. After reconstitution into proteoliposomes, the enzyme catalyzed ATP synthesis driven by an artificially induced transmembrane electrical potential (Δψ). A transmembrane proton gradient or sodium ion gradient in the absence of Δψ was not sufficient to drive ATP synthesis. ATP synthesis was eliminated by the electrogenic protonophore carbonyl cyanide m-chlorophenylhydrazone, while the electroneutral Na+/H+ antiporter monensin had no effect. Neither ATP synthesis nor ATP hydrolysis was stimulated by Na+ ions, suggesting that protons are the coupling ions of the ATP synthase from strain TA2.A1, as documented previously for mesophilic alkaliphilic Bacillus species. The ATP synthase was specifically modified at its c subunits by N,N′-dicyclohexylcarbodiimide, and this modification inhibited ATP synthesis.

Download Full-text

Meiosis-specific recombinase Dmc1 is a potent inhibitor of the Srs2 antirecombinase

Proceedings of the National Academy of Sciences ◽

10.1073/pnas.1810457115 ◽

2018 ◽

Vol 115 (43) ◽

pp. E10041-E10048 ◽

Cited By ~ 14

Author(s):

J. Brooks Crickard ◽

Kyle Kaniecki ◽

Youngho Kwon ◽

Patrick Sung ◽

Eric C. Greene

Keyword(s):

Chromosome Segregation ◽

Single Molecule ◽

Atp Hydrolysis ◽

Potent Inhibitor ◽

Chromosomal Rearrangements ◽

Motor Protein ◽

Product Formation ◽

Gross Chromosomal Rearrangements ◽

Strand Annealing ◽

Hydrolysis Activity

Cross-over recombination products are a hallmark of meiosis because they are necessary for accurate chromosome segregation and they also allow for increased genetic diversity during sexual reproduction. However, cross-overs can also cause gross chromosomal rearrangements and are therefore normally down-regulated during mitotic growth. The mechanisms that enhance cross-over product formation upon entry into meiosis remain poorly understood. In Saccharomyces cerevisiae, the Superfamily 1 (Sf1) helicase Srs2, which is an ATP hydrolysis-dependent motor protein that actively dismantles recombination intermediates, promotes synthesis-dependent strand annealing, the result of which is a reduction in cross-over recombination products. Here, we show that the meiosis-specific recombinase Dmc1 is a potent inhibitor of Srs2. Biochemical and single-molecule assays demonstrate that Dmc1 acts by inhibiting Srs2 ATP hydrolysis activity, which prevents the motor protein from undergoing ATP hydrolysis-dependent translocation on Dmc1-bound recombination intermediates. We propose a model in which Dmc1 helps contribute to cross-over formation during meiosis by antagonizing the antirecombinase activity of Srs2.

Download Full-text

Uncovering the Basis of ATP Hydrolysis Activity in Purified Human p53 Protein: A Reinvestigation

PLoS ONE ◽

10.1371/journal.pone.0093652 ◽

2014 ◽

Vol 9 (4) ◽

pp. e93652

Author(s):

Shalini Verma ◽

Basuthkar J. Rao

Keyword(s):

Atp Hydrolysis ◽

P53 Protein ◽

Protein A ◽

Hydrolysis Activity

Download Full-text

Mg2+-dependent ATP occlusion at the first nucleotide-binding domain (NBD1) of CFTR does not require the second (NBD2)

Biochemical Journal ◽

10.1042/bj20081068 ◽

2008 ◽

Vol 416 (1) ◽

pp. 129-136 ◽

Cited By ~ 14

Author(s):

Luba Aleksandrov ◽

Andrei Aleksandrov ◽

John R. Riordan

Keyword(s):

Atp Hydrolysis ◽

Nucleotide Binding ◽

Binding Pocket ◽

Atp Binding ◽

Transmembrane Conductance Regulator ◽

Transmembrane Conductance ◽

Bivalent Cation ◽

Binding Domains ◽

Rapid Hydrolysis ◽

Cystic Fibrosis Transmembrane

ATP binding to the first and second NBDs (nucleotide-binding domains) of CFTR (cystic fibrosis transmembrane conductance regulator) are bivalent-cation-independent and -dependent steps respectively [Aleksandrov, Aleksandrov, Chang and Riordan (2002) J. Biol. Chem. 277, 15419–15425]. Subsequent to the initial binding, Mg2+ drives rapid hydrolysis at the second site, while promoting non-exchangeable trapping of the nucleotide at the first site. This occlusion at the first site of functional wild-type CFTR is somewhat similar to that which occurs when the catalytic glutamate residues in both of the hydrolytic sites of P-glycoprotein are mutated, which has been proposed to be the result of dimerization of the two NBDs and represents a transient intermediate formed during ATP hydrolysis [Tombline and Senior (2005) J. Bioenerg. Biomembr. 37, 497–500]. To test the possible relevance of this interpretation to CFTR, we have now characterized the process by which NBD1 occludes [32P]N3ATP (8-azido-ATP) and [32P]N3ADP (8-azido-ADP). Only N3ATP, but not N3ADP, can be bound initially at NBD1 in the absence of Mg2+. Despite the lack of a requirement for Mg2+ for ATP binding, retention of the NTP at 37 °C was dependent on the cation. However, at reduced temperature (4 °C), N3ATP remains locked in the binding pocket with virtually no reduction over a 1 h period, even in the absence of Mg2+. Occlusion occurred identically in a ΔNBD2 construct, but not in purified recombinant NBD1, indicating that the process is dependent on the influence of regions of CFTR in addition to NBD1, but not NBD2.

Download Full-text

Transport of Alzheimer’s associated amyloid-β catalyzed by P-glycoprotein

PLoS ONE ◽

10.1371/journal.pone.0250371 ◽

2021 ◽

Vol 16 (4) ◽

pp. e0250371

Author(s):

James W. McCormick ◽

Lauren Ammerman ◽

Gang Chen ◽

Pia D. Vogel ◽

John G. Wise

Keyword(s):

Cell Culture ◽

Atp Hydrolysis ◽

Amyloid Β ◽

Md Simulations ◽

Membrane Transporter ◽

Biochemical Activity ◽

Glycoprotein P ◽

P Glycoprotein ◽

Hydrolysis Activity

P-glycoprotein (P-gp) is a critical membrane transporter in the blood brain barrier (BBB) and is implicated in Alzheimer’s disease (AD). However, previous studies on the ability of P-gp to directly transport the Alzheimer’s associated amyloid-β (Aβ) protein have produced contradictory results. Here we use molecular dynamics (MD) simulations, transport substrate accumulation studies in cell culture, and biochemical activity assays to show that P-gp actively transports Aβ. We observed transport of Aβ40 and Aβ42 monomers by P-gp in explicit MD simulations of a putative catalytic cycle. In in vitro assays with P-gp overexpressing cells, we observed enhanced accumulation of fluorescently labeled Aβ42 in the presence of Tariquidar, a potent P-gp inhibitor. We also showed that Aβ42 stimulated the ATP hydrolysis activity of isolated P-gp in nanodiscs. Our findings expand the substrate profile of P-gp, and suggest that P-gp may contribute to the onset and progression of AD.

Download Full-text

F1F0-ATP synthase from bovine heart mitochondria: development of the purification of a monodisperse oligomycin-sensitive ATPase

Biochemical Journal ◽

10.1042/bj2950799 ◽

1993 ◽

Vol 295 (3) ◽

pp. 799-806 ◽

Cited By ~ 30

Author(s):

R Lutter ◽

M Saraste ◽

H S van Walraven ◽

M J Runswick ◽

M Finel ◽

...

Keyword(s):

Atp Synthase ◽

Atp Hydrolysis ◽

Gel Filtration ◽

Primary Objective ◽

Membrane Domain ◽

Mitochondrial Membranes ◽

F1 Atpase ◽

Ammonium Sulphate Precipitation ◽

F1f0 Atp Synthase ◽

Hydrolysis Activity

A new procedure for the isolation of ATP synthase from bovine mitochondria has been developed, with the primary objective of producing enzyme suitable for crystallization trials. Proteins were extracted from mitochondrial membranes with dodecyl-beta-D-maltoside, and the ATP synthase was purified from the extract in the presence of the same detergent by a combination of ion-exchange and gel-filtration chromatography and ammonium sulphate precipitation. This simple and rapid procedure yields 20-30 mg of highly pure and monodisperse enzyme, evidently consisting of 14 different subunits, amongst them, in apparently stoichiometric amounts with the established subunits, subunit e, a recently discovered subunit of unknown function. The enzyme preparation has an oligomycin-sensitive ATP hydrolysis activity, and so the F1 domain is functionally associated with the membrane domain, F0. In contrast with the N-termini of some of the subunits of bovine mitochondrial F1-ATPase, those of the F1F0-ATP synthase are not degraded by proteolysis during the isolation procedure. This preparation therefore satisfies prerequisites for crystallization trials.

Download Full-text