Probing structurally altered and aggregated states of therapeutically relevant proteins using <scp>G</scp>roEL coupled to bio‐layer interferometry

Naik, Subhashchandra; Kumru, Ozan S.; Cullom, Melissa; Telikepalli, Srivalli; Lindboe, Elizabeth; Roop, Taylor L.; Joshi, Sangeeta B.; Amin, Divya N.; Gao, Phillip; Middaugh, C. Russell; Volkin, David B.; Fisher, Mark T.

doi:10.1002/pro.2515

Cited by 17 publications

(27 citation statements)

References 51 publications

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“…Once assembled complexes are released from the small BLI biosensor tips into small volumes (e.g., 2–3 μl), the formation of large complexes (>100 kDa) can be easily verified using electron microscopy (Fig. 9; Naik et al 2013, 2014). …”

Section: Accelerating and Validating Em Sample Preparation Of Transitmentioning

confidence: 99%

“…Furthermore, it is entirely possible that one can use EM validation of membrane protein insertion into lipid nanodiscs with small membrane proteins because insertion can be confirmed kinetically and by EM analysis. In the latter case, one could construct lipid nanodisc–small membrane protein complexes and validate the insertion of the protein into the nanodisc using specific monoclonal antibodies against the small membrane protein since antibody molecules are easily distinguished in an EM image field (Hernández-Rocamora et al 2012; Naik et al 2014). It is important to note that some commercially available MSPS that are used to form nanodiscs contain poly-histidine tags, enabling one with the ability to capture newly formed nanodiscs that can bind to Ni NTA BLI biosensor surfaces.…”

Section: Accelerating and Validating Em Sample Preparation Of Transitmentioning

confidence: 99%

“…The advantage of using this micro-scale volume release approach is obvious since it can decrease testing times for optimal complex formation and can accelerate visualization of complex formation. This particular strategy of validating complexes using micro-scale samples for EM analysis from BLI platforms has also been used to evaluate and visualize protein–protein interactions between GroEL and pre-aggregates of therapeutic proteins (Naik et al 2014). …”

Section: Accelerating and Validating Em Sample Preparation Of Transitmentioning

confidence: 99%

“…The ability to observe complex formation using label-free methods, removing the complex from these platforms, and depositing these directly onto electron microscopy grids will allow easy validation of assembly and insertion methods for scale up, eventually enabling one to rapidly generate pure samples to obtain high resolution structures (Naik et al 2013, 2014). By immobilizing and orientating soluble toxins prior to their insertion into nanodisc micelles, the crucial transition steps can be captured, allowing one to acquire high atomic resolution of toxin translocation competent states.…”

Section: Future Prospectsmentioning

confidence: 99%

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Following Natures Lead: On the Construction of Membrane-Inserted Toxins in Lipid Bilayer Nanodiscs

et al. 2015

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Bacterial toxin or viral entry into the cell often requires cell surface binding and endocytosis. The endosomal acidification induces a limited unfolding/refolding and membrane insertion reaction of the soluble toxins or viral proteins into their translocation competent or membrane inserted states. At the molecular level, the specific orientation and immobilization of the pre-transitioned toxin on the cell surface is often an important prerequisite prior to cell entry. We propose that structures of some toxin membrane insertion complexes may be observed through procedures where one rationally immobilizes the soluble toxin so that potential unfolding ↔ refolding transitions that occur prior to membrane insertion orientate away from the immobilization surface in the presence of lipid micelle pre-nanodisc structures. As a specific example, the immobilized prepore form of the anthrax toxin pore translocon or protective antigen can be transitioned, inserted into a model lipid membrane (nanodiscs), and released from the immobilized support in its membrane solubilized form. This particular strategy, although unconventional, is a useful procedure for generating pure membrane-inserted toxins in nanodiscs for electron microscopy structural analysis. In addition, generating a similar immobilized platform on label-free biosensor surfaces allows one to observe the kinetics of these acid-induced membrane insertion transitions. These platforms can facilitate the rational design of inhibitors that specifically target the toxin membrane insertion transitions that occur during endosomal acidification. This approach may lead to a new class of direct anti-toxin inhibitors.

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Section: Accelerating and Validating Em Sample Preparation Of Transitmentioning

confidence: 99%

Section: Accelerating and Validating Em Sample Preparation Of Transitmentioning

confidence: 99%

Section: Accelerating and Validating Em Sample Preparation Of Transitmentioning

confidence: 99%

Section: Future Prospectsmentioning

confidence: 99%

See 2 more Smart Citations

Following Natures Lead: On the Construction of Membrane-Inserted Toxins in Lipid Bilayer Nanodiscs

et al. 2015

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“…on a biosensor; changes in the reflected interference wave pattern between the sample and an internal reference layer result in a phase shift that can be followed in real time in both kinetic and quantitative modes [22]. All experiments were performed in kinetic buffer (20 mM PBS, pH 7.0; 1 mg/ml bovine serum albumin (BSA), and 0.02% Tween 20).…”

Section: Biolayer Interferometrymentioning

confidence: 99%

Assembly of cellulases with synthetic protein scaffolds in vitro

Gao

Ren

et al. 2015

Bioresour. Bioprocess.

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Background: Enzymatic cascades in metabolic pathways are spatially organized in such a way as to facilitate the flow of substrates. The construction of artificial cellulase complexes that mimic natural multienzyme assemblies can potentially enhance the capacity for cellulose hydrolysis. In this study, an artificial cellulase complex was constructed by tethering three cellulases to a synthetic protein scaffold. Results: Three pairs of interacting proteins were selected and characterized. The artificial protein scaffolds were constructed by fusing three interacting proteins. Cellulases were tethered to these synthetic scaffolds in different orders. The optimal assembly resulted in a 1.5-fold higher hydrolysis of cellulose than that achieved by unassembled cellulases. Conclusions: A novel artificial protein scaffold was constructed and used to assemble three cellulases. The resultant increase in enzymatic activity suggests that this can be used as a strategy for enhancing the biocatalytic capacity of enzyme cascades.

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Hydrogen Exchange Mass Spectrometry as an Emerging Analytical Tool for Stabilization and Formulation Development of Therapeutic Monoclonal Antibodies

Majumdar¹,

Middaugh²,

Weis³

et al. 2016

Hydrogen Exchange Mass Spectrometry of Proteins

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Probing structurally altered and aggregated states of therapeutically relevant proteins using GroEL coupled to bio‐layer interferometry

Cited by 17 publications

References 51 publications

Following Natures Lead: On the Construction of Membrane-Inserted Toxins in Lipid Bilayer Nanodiscs

Following Natures Lead: On the Construction of Membrane-Inserted Toxins in Lipid Bilayer Nanodiscs

Assembly of cellulases with synthetic protein scaffolds in vitro

Hydrogen Exchange Mass Spectrometry as an Emerging Analytical Tool for Stabilization and Formulation Development of Therapeutic Monoclonal Antibodies

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