Real Time Measurements of Membrane Protein:Receptor Interactions Using Surface Plasmon Resonance (SPR)

Levanon, Nurit Livnat; Vigonsky, Elena; Lewinson, Oded

doi:10.3791/51937

Cited by 7 publications

(6 citation statements)

References 9 publications

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“…Like all ABC importers BtuC 2 D 2 must associate with its cognate SBP since it is the latter that binds the substrate and delivers it to the transporter. We measured the interaction between BtuC 2 D 2 that had worked or rested at 28 °C and BtuF using Surface Plasmon Resonance 29 . We loaded identical amounts (by mass) of worked or rested BtuC 2 D 2 onto a biosensor chip and then washed the chip 50,000-fold to remove any residual ATP.…”

Section: Resultsmentioning

confidence: 99%

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The uncoupled ATPase activity of the ABC transporter BtuC2D2 leads to a hysteretic conformational change, conformational memory and improved activity

Livnat-Levanon

Gilson

Ben‐Tal

et al. 2016

Sci Rep

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ABC transporters comprise a large and ubiquitous family of proteins. From bacteria to man they translocate solutes at the expense of ATP hydrolysis. Unlike other enzymes that use ATP as an energy source, ABC transporters are notorious for having high levels of basal ATPase activity: they hydrolyze ATP also in the absence of their substrate. It is unknown what are the effects of such prolonged and constant activity on the stability and function of ABC transporters or any other enzyme. Here we report that prolonged ATP hydrolysis is beneficial to the ABC transporter BtuC2D2. Using ATPase assays, surface plasmon resonance interaction experiments, and transport assays we observe that the constantly active transporter remains stable and functional for much longer than the idle one. Remarkably, during extended activity the transporter undergoes a slow conformational change (hysteresis) and gradually attains a hyperactive state in which it is more active than it was to begin with. This phenomenon is different from stabilization of enzymes by ligand binding: the hyperactive state is only reached through ATP hydrolysis, and not ATP binding. BtuC2D2 displays a strong conformational memory for this excited state, and takes hours to return to its basal state after catalysis terminates.

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Section: Resultsmentioning

confidence: 99%

“…The procedure for measuring the interaction between BtuC 2 D 2 and BtuF using SPR had been extensively described 28 29 . Briefly, BtuC 2 D 2 (15–20 ng, 1500–2000 RU) was immobilized onto a Ni-NTA biosensor chip (GE healthcare) and FLAG-tagged BtuF was injected at the indicated concentration.…”

Section: Methodsmentioning

confidence: 99%

The uncoupled ATPase activity of the ABC transporter BtuC2D2 leads to a hysteretic conformational change, conformational memory and improved activity

Livnat-Levanon

Gilson

Ben‐Tal

et al. 2016

Sci Rep

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“…All measurements were performed using a Biacore T200 (GE Healthcare) as extensively as described before (34,35,60). His-HmuUV, His-BtuCD, and His-MolBC were immobilized directly onto nickel-nitrilotriacetic acid biosensor chip (GE Healthcare).…”

Section: Spr Measurementsmentioning

confidence: 99%

ATP binding and hydrolysis disrupt the high-affinity interaction between the heme ABC transporter HmuUV and its cognate substrate-binding protein

Qasem-Abdullah

Perach

Livnat-Levanon

et al. 2017

Journal of Biological Chemistry

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Using the energy of ATP hydrolysis, ABC transporters catalyze the trans-membrane transport of molecules. In bacteria, these transporters partner with a high-affinity substrate-binding protein (SBP) to import essential micronutrients. ATP binding by Type I ABC transporters (importers of amino acids, sugars, peptides, and small ions) stabilizes the interaction between the transporter and the SBP, thus allowing transfer of the substrate from the latter to the former. In Type II ABC transporters (importers of trace elements, vitamin B, heme, and iron-siderophores) the role of ATP remains debatable. Here we studied the interaction between the ABC heme importer (HmuUV) and its partner substrate-binding protein (HmuT). Using real-time surface plasmon resonance experiments and interaction studies in membrane vesicles, we find that in the absence of ATP the transporter and the SBP tightly bind. Substrate in excess inhibits this interaction, and ATP binding by the transporter completely abolishes it. To release the stable docked SBP from the transporter hydrolysis of ATP is required. Based on these results we propose a mechanism for heme acquisition by HmuUV-T where the substrate-loaded SBP docks to the nucleotide-free outward-facing conformation of the transporter. ATP binding leads to formation of an occluded state with the substrate trapped in the trans-membrane translocation cavity. Subsequent ATP hydrolysis leads to substrate delivery to the cytoplasm, release of the SBP, and resetting of the system. We propose that other Type II ABC transporters likely share the fundamentals of this mechanism.

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“…The sensor chip typically used in BIAcore system, that employs the Kretschmann con iguration [16,17], is a dextran matrix, composed of a thioalkane linker layer (~100 nm thick), that creates an hydrophilic environment for different chemical methods of ligand immobilization, which usually require an amount of ligand immobilized (about 10,000 RU) that corresponds to approximately ≈70 fmol/mm2, and for binding process [18]. The activation of the gold layer and the application of a speci ic coat avoid non-speci ic binding of biomolecules to the activated surface [19]. Furthermore, the dextran matrix allows both ligand immobilization with minimal conformational distortion and maximum access of the binding epitopes of ligand and analyte.…”

Section: Spr Technologymentioning

confidence: 99%

Surface Plasmon Resonance technology to assess biological interactions

Bartollino¹

2017

Insights Biol Med

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Molecular interactions between proteins or between proteins and small molecules are pivotal events for selective binding of biological structures and, consequentially, for their correct function. In this scenario, the evaluation of kinetic parameters, characterizing a molecular interactions, is considered a crucial event to reveal the nature of binding processes. The focus on peculiar forces involved in the molecular recognition represents an opportunity to explore biological interactions in real time, and to develop a number of innovative biotechnological methods for diagnosis and/or therapy. Currently, optical biosensors, offering an increasingly effective technology to detect in real time molecular binding, are usually composed by a detector, a sensor surface and a sample delivery system: only defi nite substances, which are able to interact specifi cally with the biological part, lead to an optical or electrical signal of the physical transducer. In this review we want to highlight the exponentially-growing interest of Surface Plasmon Resonance (SPR) based optical biosensors for molecular binding analysis in different research fi elds.

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Real Time Measurements of Membrane Protein:Receptor Interactions Using Surface Plasmon Resonance (SPR)

Cited by 7 publications

References 9 publications

The uncoupled ATPase activity of the ABC transporter BtuC2D2 leads to a hysteretic conformational change, conformational memory and improved activity

The uncoupled ATPase activity of the ABC transporter BtuC2D2 leads to a hysteretic conformational change, conformational memory and improved activity

ATP binding and hydrolysis disrupt the high-affinity interaction between the heme ABC transporter HmuUV and its cognate substrate-binding protein

Surface Plasmon Resonance technology to assess biological interactions

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