The interplay between bone morphogenetic proteins (BMPs) and their antagonists governs developmental and cellular processes as diverse as establishment of the embryonic dorsal-ventral axis, induction of neural tissue, formation of joints in the skeletal system and neurogenesis in the adult brain. So far, the three-dimensional structures of BMP antagonists and the structural basis for inactivation have remained unknown. Here we report the crystal structure of the antagonist Noggin bound to BMP-7, which shows that Noggin inhibits BMP signalling by blocking the molecular interfaces of the binding epitopes for both type I and type II receptors. The BMP-7-binding affinity of site-specific variants of Noggin is correlated with alterations in bone formation and apoptosis in chick limb development, showing that Noggin functions by sequestering its ligand in an inactive complex. The scaffold of Noggin contains a cystine (the oxidized form of cysteine) knot topology similar to that of BMPs; thus, ligand and antagonist seem to have evolved from a common ancestral gene.
N- and C-terminal cytoplasmic domains of inwardly rectifying K (Kir) channels control the ion-permeation pathway through diverse interactions with small molecules and protein ligands in the cytoplasm. Two new crystal structures of the cytoplasmic domains of Kir2.1 (Kir2.1(L)) and the G protein-sensitive Kir3.1 (Kir3.1(S)) channels in the absence of PIP(2) show the cytoplasmic ion-permeation pathways occluded by four cytoplasmic loops that form a girdle around the central pore (G-loop). Significant flexibility of the pore-facing G-loop of Kir2.1(L) and Kir3.1(S) suggests a possible role as a diffusion barrier between cytoplasmic and transmembrane pores. Consistent with this, mutations of the G-loop disrupted gating or inward rectification. Structural comparison shows a di-aspartate cluster on the distal end of the cytoplasmic pore of Kir2.1(L) that is important for modulating inward rectification. Taken together, these results suggest the cytoplasmic domains of Kir channels undergo structural changes to modulate gating and inward rectification.
Activins and bone morphogenetic proteins (BMPs) elicit diverse biological responses by signaling through two pairs of structurally related type I and type II receptors. Here we report the crystal structure of BMP7 in complex with the extracellular domain (ECD) of the activin type II receptor. Our structure produces a compelling four-receptor model, revealing that the types I and II receptor ECDs make no direct contacts. Nevertheless, we find that truncated receptors lacking their cytoplasmic domain retain the ability to cooperatively assemble in the cell membrane. Also, the affinity of BMP7 for its low-affinity type I receptor ECD increases 5-fold in the presence of its type II receptor ECD. Taken together, our results provide a view of the ligand-mediated cooperative assembly of BMP and activin receptors that does not rely on receptor-receptor contacts.
K + channels conduct and regulate K + flux across the cell membrane. Several crystal structures and biophysical studies of tetrameric ion channels have revealed many of the structural details of ion selectivity and gating. A narrow pore lined with four arrays of carbonyl groups is responsible for ion selectivity, whereas a conformational change of the four inner transmembrane helices (TM2) is involved in gating. We used NMR to examine full-length KcsA, a prototypical K + channel, in its open, closed and intermediate states. These studies reveal that at least two conformational states exist both in the selectivity filter and near the C-terminal ends of the TM2 helices. In the ion-conducting open state, we observed rapid structural exchange between two conformations of the filter, presumably of low and high K + affinity, respectively. Such measurements of millisecond-timescale dynamics reveal the basis for simultaneous ion selection and gating.The simplest structural definition of ion channel gating is the ability to alternate, in a signaldependent way, between states that selectively permit the flow of ions (open) or do not (closed). In the closed state, generally a default state, K + channels inhibit ion flow with high efficacy. In the open state, two opposing tasks must be carried out near the diffusion limit: ion selection and permeation 1 . Energetically, ion selection requires spatial coordination that favors K + over other cations, whereas permeation requires the rapid release of the cation from these recognition sites. This 'hold-and-release' feature underlies the unique structural and dynamical properties of the channel.Crystal structures of K + channels of prokaryotic origin (KcsA 2 , MthK 3 , KirBac1.1 (ref. 4), KvAP 5 and NaK 6 ) have revealed a universal structural framework for these tasks. To explain ion selectivity, the structures show a narrow filter composed of four successive layers of main chain carbonyl oxygen atoms, which act as surrogate waters for the dehydrated K + ions (1.35-Å radius) as they pass through the filter. This unique spatial geometry results from the signature filter amino acid sequence, Gly-Tyr-Gly, in which the two glycines enable positive φ/ψ angles of the protein backbone so that the K + -coordinating carbonyl oxygens can all point inward to the pore axis simultaneously 7 to perform ion selection 8,9 . For gating of the channel, the pore-lining C-terminal ends of the inner AUTHOR CONTRIBUTIONSK.A.B. and C.T. prepared KcsA; K.A.B., C.T., W.K. and R.R. collected and analyzed NMR data; K.A.B., C.T., S.C. and R.R. contributed to scientific discussions and prepared the manuscript. Fig. 3 online), we have obtained B85% of the sequential backbone assignments of full-length KcsA(tox) at pH 7 (Fig. 1). A residue-specific secondary structure analysis based on positive 13 Cα chemical shift deviations from a random coil (Fig. 1a), amide-H 2 O exchange ( Supplementary Fig. 4b online) and protein-detergent NOEs ( Supplementary Fig. 4a) revealed the presence of the following he...
SUMMARY HET-S (97% identical to HET-s) has an N-terminal globular domain that exerts a prion-inhibitory effect in cis on its own prion-forming domain (PFD) and in trans on HET-s prion propagation. We show that HET-S fails to form fibrils in vitro and that it inhibits HET-s PFD fibrillization in trans. In vivo analyses indicate that β-structuring of the HET-S PFD is required for HET-S activity. The crystal structures of the globular domains of HET-s and HET-S are highly similar, comprising a helical fold, while NMR-based characterizations revealed no differences in the conformations of the PFDs. We conclude that prion inhibition is not encoded by structure but rather in stability and oligomerization properties: when HET-S forms a prion seed or is incorporated into a HET-s fibril via its PFD, the β-structuring in this domain induces a change in its globular domain, generating a molecular species that is incompetent for fibril growth.
scite is a Brooklyn-based organization that helps researchers better discover and understand research articles through Smart Citations–citations that display the context of the citation and describe whether the article provides supporting or contrasting evidence. scite is used by students and researchers from around the world and is funded in part by the National Science Foundation and the National Institute on Drug Abuse of the National Institutes of Health.
hi@scite.ai
10624 S. Eastern Ave., Ste. A-614
Henderson, NV 89052, USA
Copyright © 2024 scite LLC. All rights reserved.
Made with 💙 for researchers
Part of the Research Solutions Family.