The high- and low-affinity receptor binding sites of growth hormone are allosterically coupled

Walsh, Scott T. R.; Sylvester, Juliesta E.; Kossiakoff, Anthony A.

doi:10.1073/pnas.0403336101

Cited by 32 publications

(25 citation statements)

References 27 publications

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“…This interpretation extends and strengthens the data we have previously published for hPRL (9). Additionally, Walsh et al (10) have recently described a similar allosteric coupling of the two human growth hormone receptor binding sites in hGH, suggesting that a similar mechanism may govern hGH receptor binding. We have recently identified contiguous residues in hGH (15)-and hPRL (34)-constituting motifs that, when mutated, uncouple sites 1 and 2.…”

Section: Discussionsupporting

confidence: 73%

“…Previous surface plasmon resonance and Förster resonance energy transfer (FRET) data from our laboratory indicated that receptor binding induced a conformation change in the hormone associated with a functional coupling of sites1 and 2 (9). The observation that hPRL undergoes a conformational change upon receptor binding is consistent with observations of hGH or hPL binding the extracellular domain of the hPRL receptor (10,11) or when hGH binds the extracellular domain of the hGH receptor (12,13). The idea that the receptor binding events are functionally coupled also is consistent with the positive 1.7 Hill coefficient described by Hooper et al (3) in a heterologous ovine PRL/rat PRL receptor system.…”

supporting

confidence: 76%

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Obligate Ordered Binding of Human Lactogenic Cytokines

Voorhees

Brooks

2010

Journal of Biological Chemistry

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Class 1 cytokines bind two receptors to create an active heterotrimeric complex. It has been argued that ligand binding to their receptors is an ordered process, but a structural mechanism describing this process has not been determined. We have previously described an obligate ordered binding mechanism for the human prolactin/prolactin receptor heterotrimeric complex. In this work we expand this conceptual understanding of ordered binding to include three human lactogenic hormones: prolactin, growth hormone, and placental lactogen. We independently blocked either of the two receptor binding sites of each hormone and used surface plasmon resonance to measure human prolactin receptor binding kinetics and stoichiometries to the remaining binding surface. When site 1 of any of the three hormones was blocked, site 2 could not bind the receptor. But blocking site 2 did not affect receptor binding at site 1, indicating a requirement for receptor binding to site 1 before site 2 binding. In addition we noted variable responses to the presence of zinc in hormone-receptor interaction. Finally, we performed Förster resonance energy transfer (FRET) analyses where receptor binding at subsaturating stoichiometries induced changes in FRET signaling, indicative of binding-induced changes in hormone conformation, whereas at receptor: hormone ratios in excess of 2:1 no additional changes in FRET signaling were observed. These results strongly support a conformationally mediated obligate-ordered receptor binding for each of the three lactogenic hormones.Human prolactin (hPRL), 2 growth hormone (hGH), and placental lactogen (hPL) are hormones belonging to the class 1 cytokine family (1). These three proteins share significant sequence homologies; the more closely related hPL and hPRL display 85% sequence identity, and hPRL shares a 23% identity with hGH. Each of these four-helix bundle proteins is recognized as a lactogenic hormone based on their ability to bind and activate primate prolactin receptors (2). The binding reaction that takes place between lactogenic hormones and the prolactin receptor results in the formation of a heterotrimeric complex with a 2:1 ratio of receptor to hormone (3) (Fig. 1). The formation of this ternary complex is believed to proceed in an ordered process in which the N-terminal S1 subdomain of the prolactin receptor first binds at a hormone surface comprised of elements of helices 1 and 4 as well as the sequence connecting helices 1 and 2 (site 1) before subsequently binding a second prolactin receptor by its S1 subdomain at a hormone surface composed of elements of helices 1 and 3 (site 2). During secondary receptor binding, an additional receptor-receptor binding surface is formed between the C-terminal S2 subdomains of the membrane-bound receptors and is distal to the bound hormone. Thus, for site 2 the ⌬G is divided between the hormone/ receptor interfaces and the two interacting S2 receptor surfaces. The formation of this extracellular trimolecular complex orients the intracellular domains of the...

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Section: Discussionsupporting

confidence: 73%

supporting

confidence: 76%

Obligate Ordered Binding of Human Lactogenic Cytokines

Voorhees

Brooks

2010

Journal of Biological Chemistry

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“…However, no detailed molecular mechanism was formulated, and the extent to which PRL actually undergoes significant structural rearrangements when interacting with the receptor chain via BS1 has been a matter of some debate. In the GH system, it has been demonstrated that BS1 and BS2 are allosterically coupled in the sense that mutations in BS1 can induce conformational changes in BS2 (35). The recent publication of the crystal structure of the PRLR antagonist, PRLv3 (16), in combination with the present determination of the receptor-complexed structure of the closely related variant, PRLv2, provides a unique opportunity to scrutinize the structural rearrangements associated with receptor binding at BS1.…”

Section: Discussionmentioning

confidence: 99%

Crystal Structure of a Prolactin Receptor Antagonist Bound to the Extracellular Domain of the Prolactin Receptor

Svensson

Bondensgaard

Nørskov-Lauritsen

et al. 2008

Journal of Biological Chemistry

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The crystal structure of the complex between an N-terminally truncated G129R human prolactin (PRL) variant and the extracellular domain of the human prolactin receptor (PRLR) was determined at 2.5 Å resolution by x-ray crystallography. This structure represents the first experimental structure reported for a PRL variant bound to its cognate receptor. The binding of PRL variants to the PRLR extracellular domain was furthermore characterized by the solution state techniques, hydrogen exchange mass spectrometry, and NMR spectroscopy. Compared with the binding interface derived from mutagenesis studies, the structural data imply that the definition of PRL binding site 1 should be extended to include residues situated in the N-terminal part of loop 1 and in the C terminus. Prolactin (PRL)4 is a protein hormone secreted by the anterior pituitary in vertebrates and possesses physiological functions of remarkable diversity, including effects on reproduction, lactation, and growth. PRL belongs to a family of homologous proteins comprising PRL, growth hormone (GH), and placental lactogen (PL). The biological effects associated with this cytokine family are mediated by two distinct classes of cell surface receptors, the PRL receptors (PRLR) and the GH receptors (GHR). The PRL/PL/GH biology is governed by a delicate balance between receptor cross-reactivity and selectivity; PRL and PL bind selectively to PRLR, whereas GH is capable of binding both PRLR and GHR.After being proposed more than a decade ago (1), hormoneinduced receptor dimerization became generally accepted as the model for cytokine receptor activation. For the PRL family members, the model describes the signaling molecular entity as a ternary complex between one hormone molecule and a receptor homodimer assembled in a strictly sequential and hormonedependent fashion; first the hormone ligand engages via binding site 1 (BS1) in high affinity binding to one receptor chain forming a 1:1 hormone-receptor complex. This complex constitutes the template for binding a second, identical receptor molecule via binding site 2 (BS2), resulting in the active 1:2 complex. However, the model has been challenged by an increasing body of experimental evidence, initially reported for the homologous human erythropoietin receptor (2) and later for GHR (3) and PRLR (4). These studies suggest that preformed, inactive dimers exist in the absence of hormone. Thus, receptor dimerization is a necessary but not sufficient event for receptor activation and, notably, not strictly ligand-dependent. For both human erythropoietin receptor (5) and GHR (3), mechanistic models have been proposed, where receptor activation involves relative rotations and movements of receptor subunits induced by hormone binding. Allosteric reorganization of the intracellular receptor domains brings associated JAK2 kinases into close proximity, allowing their activation by cross-phosphorylation. This initial activation step triggers a cascade of molecular events leading to the functional receptor response (6).The...

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“…Receptor homodimerization by the human growth hormone (hGH) has been shown to be allosterically regulated (37) and may represent an intermediate on such a continuum. The binding of the two receptor molecules to hGH occurs in a regulated and sequential manner.…”

Section: The Protein Core As a Potential Regulator Of Cooperativity Bmentioning

confidence: 99%

Long-range cooperative binding effects in a T cell receptor variable domain

Moza

Buonpane

Zhu

et al. 2006

Proc. Natl. Acad. Sci. U.S.A.

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Although cellular processes depend on protein-protein interactions, our understanding of molecular recognition between proteins remains far from comprehensive. Protein-protein interfaces are structural and energetic mosaics in which a subset of interfacial residues, called hot spots, contributes disproportionately to the affinity of the complex. These hot-spot residues can be further clustered into hot regions. It has been proposed that binding energetics between residues within a hot region are cooperative, whereas those between hot regions are strictly additive. If this idea held true for all protein-protein interactions, then energetically significant long-range conformational effects would be unlikely to occur. In the present study, we show cooperative binding energetics between distinct hot regions that are separated by >20 Å. Using combinatorial mutagenesis and surface plasmon resonance binding analysis to dissect additivity and cooperativity in a complex formed between a variable domain of a T cell receptor and a bacterial superantigen, we find that combinations of mutations from each of two hot regions exhibited significant cooperative energetics. Their connecting sequence is composed primarily of a single ␤-strand of the T cell receptor variable Ig domain, which has been observed to undergo a strand-switching event and does not form an integral part of the stabilizing core of this Ig domain. We propose that these cooperative effects are propagated through a dynamic structural network. Cooperativity between hot regions has significant implications for the prediction and inhibition of protein-protein interactions.binding energy ͉ cooperativity ͉ protein-protein interaction ͉ surface plasmon resonance ͉ T cell activity

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The high- and low-affinity receptor binding sites of growth hormone are allosterically coupled

Cited by 32 publications

References 27 publications

Obligate Ordered Binding of Human Lactogenic Cytokines

Obligate Ordered Binding of Human Lactogenic Cytokines

Crystal Structure of a Prolactin Receptor Antagonist Bound to the Extracellular Domain of the Prolactin Receptor

Long-range cooperative binding effects in a T cell receptor variable domain

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