Your search keyword '"Gestwicki JE"' showing total 5 results

1. Luminescence complementation assay for measurement of binding to protein C-termini in live cells.

Author

Nadel CM, Ran X, and Gestwicki JE

Subjects

HEK293 Cells, HSP70 Heat-Shock Proteins genetics, Humans, Protein Binding, Protein Domains, Ubiquitin-Protein Ligases genetics, HSP70 Heat-Shock Proteins metabolism, Luminescence, Ubiquitin-Protein Ligases metabolism

Abstract

Protein-protein interactions (PPIs) involving the extreme C-terminus serve important scaffolding and regulatory functions. Here, we leveraged NanoBiT technology to build a luminescent complementation assay for use in studying this subcategory of PPI. As a model system, we fused one component of NanoBiT to the disordered C-terminus of heat shock protein (Hsp70) and the other to its binding partner, the tetratricopeptide repeat (TPR) domain of CHIP/STUB1. We found that HEK293 cells that stably express these chimeras under a doxycycline promoter produced a robust luminescence signal. This signal was sensitive to mutations and it was further tuned by the expression of competitive C-termini. Using this system, we identified a promising, membrane permeable inhibitor of the Hsp70-CHIP interaction. More broadly, we anticipate that NanoBiT is well-suited for studying PPIs that involve C-termini., (Copyright © 2020 Elsevier Inc. All rights reserved.)

Published

2020

2. Bicinchoninic acid (BCA) assay in low volume.

Author

Bainor A, Chang L, McQuade TJ, Webb B, and Gestwicki JE

Subjects

Coloring Agents chemistry, Linear Models, Sensitivity and Specificity, Colorimetry methods, Proteins analysis, Quinolines chemistry

Abstract

The BCA assay is a colorimetric method for estimating protein concentration. In 96-well plates, the relationship between protein content and absorbance is nearly linear over a wide range; however, performance is reduced in lower volume. To overcome this limitation, we performed the BCA assays in opaque, white 384-well plates. These plates emit fluorescence between 450-600 nm when excited at 430 nm; thus, their fluorescence is quenched by the BCA chromophore (λ(max) 562 nm). This arrangement allowed accurate determination of protein content using only 2 μL of sample. Moreover, soluble flourescein could replace the white plates, creating a homogenous format., (Copyright © 2010 Elsevier Inc. All rights reserved.)

Published

2011

3. Identification of small molecules that modify the protein folding activity of heat shock protein 70.

Author

Wisén S and Gestwicki JE

Subjects

Adenosine Triphosphate metabolism, Chemistry Techniques, Analytical instrumentation, HSP40 Heat-Shock Proteins metabolism, Luciferases, Firefly metabolism, Protein Renaturation drug effects, Sensitivity and Specificity, Drug Evaluation, Preclinical, HSP70 Heat-Shock Proteins metabolism, Protein Folding, Small Molecule Libraries pharmacology

Abstract

Molecular chaperones, such as heat shock protein 70 (Hsp70) and its bacterial ortholog DnaK, play numerous important roles in protein folding. In vitro, this activity can be observed by incubating purified chaperones with denatured substrates and measuring the recovery of properly folded protein. In an effort to rapidly identify small molecules that modify this folding activity, we modified an existing method for use in 96-well plates. In this assay, denatured firefly luciferase was treated with a mixture of DnaK and prospective chemical modulators. The luminescence of refolded luciferase was used to follow the reaction progress, and counterscreens excluded compounds that target luciferase; thus, hits from these screens modify protein folding via their effects on the function of the chaperone machine. Using this platform, we screened a pilot chemical library and found five new inhibitors of DnaK and one compound that promoted folding. These chemical probes may be useful in studies aimed at understanding the many varied roles of chaperones in cellular protein folding. Moreover, this assay provides the opportunity to rapidly screen for additional compounds that might regulate the folding activity of Hsp70.

Published

2008

4. High-throughput screen for small molecules that modulate the ATPase activity of the molecular chaperone DnaK.

Author

Chang L, Bertelsen EB, Wisén S, Larsen EM, Zuiderweg ER, and Gestwicki JE

Subjects

Adenosine Triphosphatases genetics, Adenosine Triphosphate metabolism, Bacterial Proteins metabolism, Colorimetry, Escherichia coli genetics, Escherichia coli Proteins genetics, HSP70 Heat-Shock Proteins genetics, Heat-Shock Proteins metabolism, Kinetics, Recombinant Proteins metabolism, Adenosine Triphosphatases metabolism, Escherichia coli enzymology, Escherichia coli Proteins metabolism, HSP70 Heat-Shock Proteins metabolism

Abstract

DnaK is a molecular chaperone of Escherichia coli that belongs to a family of conserved 70-kDa heat shock proteins. The Hsp70 chaperones are well known for their crucial roles in regulating protein homeostasis, preventing protein aggregation, and directing subcellular traffic. Given the complexity of functions, a chemical method for controlling the activities of these chaperones might provide a useful experimental tool. However, there are only a handful of Hsp70-binding molecules known. To build this area, we developed a robust, colorimetric, high-throughput screening (HTS) method in 96-well plates that reports on the ATPase activity of DnaK. Using this approach, we screened a 204-member focused library of molecules that share a dihydropyrimidine core common to known Hsp70-binding leads and uncovered seven new inhibitors. Intriguingly, the candidates do not appear to bind the hydrophobic groove that normally interacts with peptide substrates. In sum, we have developed a reliable HTS method that will likely accelerate discovery of small molecules that modulate DnaK/Hsp70 function. Moreover, because this family of chaperones has been linked to numerous diseases, this platform might be used to generate new therapeutic leads.

Published

2008

5. Selective immobilization of multivalent ligands for surface plasmon resonance and fluorescence microscopy.

Author

Gestwicki JE, Cairo CW, Mann DA, Owen RM, and Kiessling LL

Subjects

Amines metabolism, Carboxylic Acids metabolism, Cell Adhesion physiology, Dextrans metabolism, Humans, Jurkat Cells, Ligands, Selectins metabolism, Microscopy, Fluorescence, Surface Plasmon Resonance

Abstract

Cell surface multivalent ligands, such as proteoglycans and mucins, are often tethered by a single attachment point. In vitro, however, it is difficult to immobilize multivalent ligands at single sites due to their heterogeneity. Moreover, multivalent ligands often lack a single group with reactivity orthogonal to other functionality in the ligand. Biophysical analyses of multivalent ligand-receptor interactions would benefit from the availability of strategies for uniform immobilization of multivalent ligands. To this end, we report the design and synthesis of a multivalent ligand that has a single terminal orthogonal functional group and we demonstrate that this material can be selectively immobilized onto a surface suitable for surface plasmon resonance (SPR) experiments. The polymeric ligand we generated displays multiple copies of 3,6-disulfogalactose, and it can bind to the cell adhesion molecules P- and L-selectin. Using SPR measurements, we found that surfaces displaying our multivalent ligands bind specifically to P- and L-selectin. The affinities of P- and L-selectin for surfaces displaying the multivalent ligand are five- to sixfold better than the affinities for a surface modified with the corresponding monovalent ligand. In addition to binding soluble proteins, surfaces bearing immobilized polymers bound to cells displaying L-selectin. Cell binding was confirmed by visualizing adherent cells by fluorescence microscopy. Together, our results indicate that synthetic surfaces can be created by selective immobilization of multivalent ligands and that these surfaces are capable of binding soluble and cell-surface-associated receptors with high affinity., (Copyright 2002 Elsevier Science (USA).)

Published

2002