236 research outputs found
Cryo-EM structure of the prothrombin-prothrombinase complex
The intrinsic and extrinsic pathways of the coagulation cascade converge to a common step where the prothrombinase complex, comprising the enzyme factor Xa (fXa), the cofactor fVa, Ca2+ and phospholipids, activates the zymogen prothrombin to the protease thrombin. The reaction entails cleavage at 2 sites, R271 and R320, generating the intermediates prethrombin 2 and meizothrombin, respectively. The molecular basis of these interactions that are central to hemostasis remains elusive. We solved 2 cryogenic electron microscopy (cryo-EM) structures of the fVa-fXa complex, 1 free on nanodiscs at 5.3-Å resolution and the other bound to prothrombin at near atomic 4.1-Å resolution. In the prothrombin-fVa-fXa complex, the Gla domains of fXa and prothrombin align on a plane with the C1 and C2 domains of fVa for interaction with membranes. Prothrombin and fXa emerge from this plane in curved conformations that bring their protease domains in contact with each other against the A2 domain of fVa. The 672ESTVMATRKMHDRLEPEDEE691 segment of the A2 domain closes on the protease domain of fXa like a lid to fix orientation of the active site. The 696YDYQNRL702 segment binds to prothrombin and establishes the pathway of activation by sequestering R271 against D697 and directing R320 toward the active site of fXa. The cryo-EM structure provides a molecular view of prothrombin activation along the meizothrombin pathway and suggests a mechanism for cleavage at the alternative R271 site. The findings advance our basic knowledge of a key step of coagulation and bear broad relevance to other interactions in the blood
Ground State Destabilization from a Positioned General Base in the Ketosteroid Isomerase Active Site
High-Throughput Genotyping for a Polymorphism Linked to Soybean Cyst Nematode Resistance Gene \u3ci\u3eRhg4\u3c/i\u3e by Using TaqMan\u3csup\u3eTM\u3c/sup\u3e Probes
An individual soybean breeder can generate over one hundred thousand new genotypes each year. The efficiency of selection in these populations could be improved if these genotypes were effectively screened with one DNA marker that identified an important gene, and if laboratory throughput was high and costs were low. Our aim was to develop a rapid genotyping procedure for resistance to the soybean cyst nematode. A high-throughput genotyping method was developed with fluorogenic probes to distinguish between two insertion polymorphisms in alleles of an AFLP marker that is located about 50 kbp from the Rhg4 gene candidate. The assay uses the 50 exonuclease activity of Taq polymerase in conjunction with fluorogenic probes for each allele. The method can be used for scoring the polymorphism in a recombinant inbred line population and for screening parent lines in a breeding program. The TaqManTM method of determining genotype was accurate in 90% of scores in the RIL population compared to 95% accuracy with electrophoresis. Among 94 cultivars that are parents in our breeding program allele 2 that is derived from the sources of resistance to SCN was common in resistant cultivars (30 of 56) but rare in susceptible cultivars (3 of 38). Therefore, this method can be applied to automated large-scale genotyping for soybean breeding programs
Sclerotiamide: The First Non-Peptide-Based Natural Product Activator of Bacterial Caseinolytic Protease P
Caseinolytic protease P (ClpP) maintains
essential roles in bacterial
homeostasis. As such, both the inhibition and activation of this enzyme
result in bactericidal activity, making ClpP a promising target for
antibacterial drug development. Herein, we report the results of a
fluorescence-based screen of ∼450 structurally diverse fungal
and bacterial secondary metabolites. Sclerotiamide (<b>1</b>), a paraherquamide-related indolinone, was identified as the first
non-peptide-based natural product activator of ClpP. Structure-activity
relationships arising from the initial screen, preliminary biochemical
evaluation of <b>1</b>, and rationale for the exploitation of
this chemotype to develop novel ClpP activators are presented
Ground State Destabilization from a Positioned General Base in the Ketosteroid Isomerase Active Site
We compared the binding affinities of ground state analogues
for
bacterial ketosteroid isomerase (KSI) with a wild-type anionic Asp
general base and with uncharged Asn and Ala in the general base position
to provide a measure of potential ground state destabilization that
could arise from the close juxtaposition of the anionic Asp and hydrophobic
steroid in the reaction’s Michaelis complex. The analogue binding
affinity increased ∼1 order of magnitude for the Asp38Asn mutation
and ∼2 orders of magnitude for the Asp38Ala mutation, relative
to the affinity with Asp38, for KSI from two sources. The increased
level of binding suggests that the abutment of a charged general base
and a hydrophobic steroid is modestly destabilizing, relative to a
standard state in water, and that this destabilization is relieved
in the transition state and intermediate in which the charge on the
general base has been neutralized because of proton abstraction. Stronger
binding also arose from mutation of Pro39, the residue adjacent to
the Asp general base, consistent with an ability of the Asp general
base to now reorient to avoid the destabilizing interaction. Consistent
with this model, the Pro mutants reduced or eliminated the increased
level of binding upon replacement of Asp38 with Asn or Ala. These
results, supported by additional structural observations, suggest
that ground state destabilization from the negatively charged Asp38
general base provides a modest contribution to KSI catalysis. They
also provide a clear illustration of the well-recognized concept that
enzymes evolve for catalytic function and not, in general, to maximize
ground state binding. This ground state destabilization mechanism
may be common to the many enzymes with anionic side chains that deprotonate
carbon acids
Determination of Hydrogen Bond Structure in Water versus Aprotic Environments To Test the Relationship Between Length and Stability
Hydrogen
bonds profoundly influence the architecture and activity
of biological macromolecules. Deep appreciation of hydrogen bond contributions
to biomolecular function thus requires a detailed understanding of
hydrogen bond structure and energetics and the relationship between
these properties. Hydrogen bond formation energies (Δ<i>G</i><sub><i>f</i></sub>) are enormously more favorable
in aprotic solvents than in water, and two classes of contributing
factors have been proposed to explain this energetic difference, focusing
respectively on the isolated and hydrogen-bonded species: (I) water
stabilizes the dissociated donor and acceptor groups much better than
aprotic solvents, thereby reducing the driving force for hydrogen
bond formation; and (II) water lengthens hydrogen bonds compared to
aprotic environments, thereby decreasing the potential energy within
the hydrogen bond. Each model has been proposed to provide a dominant
contribution to Δ<i>G</i><sub><i>f</i></sub>, but incisive tests that distinguish the importance of these contributions
are lacking. Here we directly test the structural basis of model II.
Neutron crystallography, NMR spectroscopy, and quantum mechanical
calculations demonstrate that O–H···O hydrogen
bonds in crystals, chloroform, acetone, and water have nearly identical
lengths and very similar potential energy surfaces despite Δ<i>G</i><sub><i>f</i></sub> differences >8 kcal/mol
across
these solvents. These results rule out a substantial contribution
from solvent-dependent differences in hydrogen bond structure and
potential energy after association (model II) and thus support the
conclusion that differences in hydrogen bond Δ<i>G</i><sub><i>f</i></sub> are predominantly determined by solvent
interactions with the dissociated groups (model I). These findings
advance our understanding of universal hydrogen-bonding interactions
and have important implications for biology and engineering
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