Name: defining hsp33's redox-regulated chaperone activity and mapping conformational changes on hsp33 using hydrogen-deuterium exchange mass spectrometry
Uploaded: 2018-06-07T15:00:00
Description: Watch this Scientific Journal Video about Defining Hsp33's Redox-regulated Chaperone Activity and Mapping Conformational Changes on Hsp33 Using Hydrogen-deuterium Exchange Mass Spectrometry at JoVE.co

The authors are thankful to Meytal Radzinski for her helpful discussions and critical reading of the article, and to Patrick Griffin and his lab members for their unlimited assistance while establishing the HDX analysis platform. The authors are grateful to the German-Israel Foundation (I-2332-1149.9/2012), the Binational Science Foundation (2015056), the Marie-Curie integration grant (618806), the Israel Science Foundation (1765/13 and 2629/16), and the Human Frontier Science Program (CDA00064/2014) for their financial support.

1. Preparation of Fully Reduced and Fully Oxidized Proteins
<ol>
	<li>Preparation of a fully reduced protein 
	Note: Here, we describe the reduction of a zinc-containing protein, and use a ZnCl2 solution to restore the Zn-incorporated, reduced protein state. The ZnCl2 solution can be replaced or discarded. Note that the time and temperature of the reduction process depends on the protein stability and function, and is thus specific per protein.
	<ol>
		<li>Thaw the protein sa...

In this paper, we provided protocols for the analysis of redox-dependent chaperone activity and the characterization of structural changes upon the binding of a client protein. These are complementary methodologies to define potential chaperone-substrate complexes and analyze potential interaction sites.
Here, we applied these protocols for the characterization of a complex between the redox-regulated chaperone Hsp33 with a well-studied chaperone substrate CS. We presented two different types ...

Cells frequently encounter an accumulation of reactive oxygen species (ROS) produced as byproducts of respiration1,2, protein and lipid oxidation3,4, and additional processes5,6,7. Despite ROS&#39; beneficial role in diverse biological processes such as cellular signaling8,9 and immune response10, an imbalance between ROS production and its detoxification might occur, leading to oxidative stress7. The biological targets of ROS are proteins, lipids, and nucleic acids, the oxidation of which affect their structure and function. Therefore, the accumulation of cellular oxidants is strongly linked to a diverse range of pathologies including cancer9,11, inflammation12,13, and aging14,15, and have been found to be involved in the onset and progression of neurodegenerative disorders such as Alzheimer&#39;s, Parkinson&#39;s, and ALS disease16,17,18.
Both newly synthesized and mature proteins are highly sensitive to oxidation due to the potentially harmful modifications of their side chains, which shape protein structure and function19,20. Therefore, oxidative stress usually leads to a widespread protein inactivation, misfolding and aggregation, eventually leading to cell death. One of the elegant cellular strategies to cope with the potential damage of protein oxidation is to utilize redox-dependent chaperones, which inhibit the widespread protein aggregation, instead of forming stable complexes with misfolded client proteins21,22,23. These first-line defense chaperones are rapidly activated by a site-specific oxidation (usually on cysteine residues) that converts them into potent anti-aggregation molecules24. Since oxidative stress results in the inhibition of respiration and in decreases in the cellular ATP levels25, canonical ATP-dependent chaperones are less effective during oxidative stress conditions25,26,27. Therefore, redox-activated ATP-independent chaperones play a vital role in maintaining protein homeostasis upon the accumulation of oxidants in bacteria and eukaryotes (e.g., Hsp3328 and RidA29 in bacteria, Get330 in yeast, peroxiredoxins31 in eukaryotes). The activity of these chaperones strongly depends on reversible structural conformational changes induced by a site-specific oxidation that uncovers hydrophobic regions involved in the recognition of misfolded client proteins.
Research of the anti-aggregation mechanism and the principles governing the recognition of the client proteins by chaperones is not easy due to the dynamic and heterogenic nature of chaperone-substrate interactions32,33,34,35,36,37. However, stress-regulated chaperones have an opportunity to advance our understanding of the anti-aggregation function due to their ability to: 1) obtain two different forms of the chaperone, active (e.g., oxidized) and inactive (e.g., reduced), with the introduction or removal of a stress condition easily switching between them (e.g., oxidant and reducing agent), 2) have a broad range of substrates, 3) form highly stable complexes with the client proteins that may be evaluated by different structural methodologies, and 4) focus solely on the substrate recognition and release, mediated by redox-dependent conformational changes, as the majority of these chaperones lacks the folding capability.
Here, we analyze the bacterial redox-regulated chaperone Hsp33&#39;s anti-aggregation activity, a vital component of the bacterial defense system against oxidation-induced protein aggregation28. When reduced, Hsp33 is a tightly folded zinc-binding protein with no chaperone activity; however, when exposed to oxidative stress, Hsp33 undergoes extensive conformational changes which expose its substrate binding regions38,39. Upon oxidation, the zinc ion that is strongly bound to four highly conserved cysteine residues of the C-terminal domain is released40. This results in the formation of two disulfide bonds, an unfolding of the C-terminal domain, and a destabilization of the adjacent linker region41. The C-terminal and linker regions are highly flexible and are defined as intrinsically or partially disordered. Upon return to non-stress conditions, the cysteines become reduced and the chaperone returns to its native folded state with no anti-aggregation activity. The refolding of the chaperone leads to a further unfolding and destabilization of the bound client protein, which triggers its transfer to the canonical chaperone system, DnaK/J, for refolding38. Analysis of Hsp33&#39;s interaction sites suggests that Hsp33 uses both its charged disordered regions as well as the hydrophobic regions on the linker and N-terminal domain to capture misfolded client proteins and prevent their aggregation38,42. In the folded state, these regions are hidden by the folded linker and C-terminal domain. Interestingly, the linker region serves as a gatekeeper of Hsp33&#39;s folded and inactive state, &#34;sensing&#34; the folding status of its adjacent C-terminal domain34. Once destabilized by mutagenesis (either by a point mutation or a full sequence perturbation), Hsp33 is converted to a constitutively active chaperone regardless the redox state of its redox-sensitive cysteines43.
The protocols presented here allow monitoring of Hsp33&#39;s redox-dependent chaperone activity, as well as mapping conformational changes upon the activation and binding of client proteins. This methodology can be adapted to research other chaperone-client recognition models as well as non-chaperone protein-protein interactions. Moreover, we present protocols for the preparation of fully reduced and oxidized chaperones that can be used in studies of other redox-switch proteins, to reveal potential roles of protein oxidation on the protein activity.
Specifically, we describe a procedure to monitor chaperone activity in vitro and define its substrate specificity under different types of protein aggregation (chemically or thermally induced) using light scattering (LS) measured by a fluorospectrometer44. During aggregation, light scattering at 360 nm increases rapidly due to the increasing turbidity. Thus, aggregation can be monitored in a time-dependent manner at this wavelength. LS is a fast and sensitive method for testing protein aggregation and thus the anti-aggregation activity of a protein of interest using nanomolar concentrations, enabling the characterization of protein aggregation-related kinetic parameters under different conditions. Moreover, the LS protocol described here does not require expensive instrumentation, and can be easily established in any laboratory.
Nevertheless, it is quite challenging to obtain &#34;clean&#34; kinetic curves and to derive a protein&#39;s kinetic parameters from such light scattering experiments, due to noise and the large number of outliers generated by air bubbles and large aggregates. To overcome this obstacle, we present a novel graphical tool, Kfits45, used for reducing noise levels in different kinetic measurements, specifically fitted for protein aggregation kinetic data. This software provides preliminary kinetic parameters for an early assessment of the results and allows the user to &#34;clean&#34; large quantities of data quickly without affecting its kinetic properties. Kfits is implemented in Python and available in open source at 45.
One of the challenging questions in the field relates to mapping interaction sites between chaperones and their client proteins and understanding how chaperones recognize a wide range of misfolded substrates. This question is further complicated when studying highly dynamic protein complexes which involve intrinsically disordered chaperones and aggregation-prone substrates. Fortunately, structural mass spectrometry has dramatically advanced over the last decade and has successfully provided helpful approaches and tools to analyze the structural plasticity and map residues involved in protein recognition46,47,48,49. Here, we present one such technique-hydrogen-deuterium exchange mass spectrometry (HDX-MS)-which allows the mapping of residue-level changes in a structural conformation upon protein modification or protein/Ligand binding35,50,51,52,53,54,55. HDX-MS uses the continuous exchange of backbone hydrogens by deuterium, the rate of which is affected by the chemical environment, accessibility, and covalent and non-covalent bonds56. HDX-MS tracks these exchange processes using a deuterated solvent, commonly heavy water (D2O), and allows measurement based on the change in molecular weight following the hydrogen to deuterium exchange. Slower rates of hydrogen-deuterium exchange can result from hydrogens participating in hydrogen bonds or, simply, from steric hindrance, which indicates local changes in structure57. Changes upon a ligand binding or post-translational modifications can also lead to differences in the hydrogen environment, with a binding resulting in differences in the hydrogen-deuterium exchange (HDX) rates46,53.
We applied this technology to 1) map Hsp33 regions which rapidly unfold upon oxidation, leading to the activation of Hsp33, and 2) define the potential binding interface of Hsp33 with its full-length misfolded substrate, citrate synthase (CS)38.
The methods described in this manuscript can be applied to study redox-dependent functions of proteins in vitro, defining anti-aggregation activity and the role of structural changes (if any) in protein function. These methodologies can be easily adapted to diverse biological systems and applied in the laboratory.

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			<td>http://kfits.reichmannlab.com/fitter/</td>
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defining hsp33's redox-regulated chaperone activity and mapping conformational changes on hsp33 using hydrogen-deuterium exchange mass spectrometry

Living organisms regularly need to cope with fluctuating environments during their life cycle, including changes in temperature, pH, the accumulation of reactive oxygen species, and more. These fluctuations can lead to a widespread protein unfolding, aggregation, and cell death. Therefore, cells have evolved a dynamic and stress-specific network of molecular chaperones, which maintain a "healthy" proteome during stress conditions. ATP-independent chaperones constitute one major class of molecular chaperones, which serve as first-line defense molecules, protecting against protein aggregation in a stress-dependent manner. One feature these chaperones have in common is their ability to utilize structural plasticity for their stress-specific activation, recognition, and release of the misfolded client. 
In this paper, we focus on the functional and structural analysis of one such intrinsically disordered chaperone, the bacterial redox-regulated Hsp33, which protects proteins against aggregation during oxidative stress. Here, we present a toolbox of diverse techniques for studying redox-regulated chaperone activity, as well as for mapping conformational changes of the chaperone, underlying its activity. Specifically, we describe a workflow which includes the preparation of fully reduced and fully oxidized proteins, followed by an analysis of the chaperone anti-aggregation activity in vitro using light-scattering, focusing on the degree of the anti-aggregation activity and its kinetics. To overcome frequent outliers accumulated during aggregation assays, we describe the usage of Kfits, a novel graphical tool which allows easy processing of kinetic measurements. This tool can be easily applied to other types of kinetic measurements for removing outliers and fitting kinetic parameters. To correlate the function with the protein structure, we describe the setup and workflow of a structural mass spectrometry technique, hydrogen-deuterium exchange mass spectrometry, that allows the mapping of conformational changes on the chaperone and substrate during different stages of Hsp33 activity. The same methodology can be applied to other protein-protein and protein-ligand interactions.

The two methods presented make it possible to follow the kinetic activity and dynamics of protein interactions between a chaperone and its substrate. Moreover, the reduction-oxidation protocol allows the preparation of a fully reduced and fully oxidized chaperone, giving a more in-depth understanding of the activation mechanism of redox-dependent disordered chaperones.
First, we used light scattering in order to examine the redo...

Watch this Scientific Journal Video about Defining Hsp33's Redox-regulated Chaperone Activity and Mapping Conformational Changes on Hsp33 Using Hydrogen-deuterium Exchange Mass Spectrometry at JoVE.co

Defining Hsp33's Redox-regulated Chaperone Activity and Mapping Conformational Changes on Hsp33 Using Hydrogen-deuterium Exchange Mass Spectrometry

One of the most challenging stress conditions that organisms encounter during their lifetime involves the accumulation of oxidants. During oxidative stress, cells heavily rely on molecular chaperones. Here, we present methods used to investigate the redox-regulated anti-aggregation activity, as well as to monitor structural changes governing the chaperone function using HDX-MS.

Living organisms regularly need to cope with fluctuating environments during their life cycle, including changes in temperature, pH, the accumulation of ...

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