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1. Phage vs. Phage: Direct Selections of Sandwich Binding Pairs

Author

Sanders, Emily C, Santos, Alicia M, Nguyen, Eugene K, Gelston, Aidan A, Majumdar, Sudipta, and Weiss, Gregory A

Subjects
Microbiology, Biological Sciences, Biotechnology, Peptide Library, Enzyme-Linked Immunosorbent Assay, Bacteriophages, Antibodies, Peptides, Biomarkers, phage display, sandwich binding, biomarker diagnostics, enzyme-linked immunosorbent assay
Abstract

The sandwich format immunoassay is generally more sensitive and specific than more common assay formats, including direct, indirect, or competitive. A sandwich assay, however, requires two receptors to bind non-competitively to the target analyte. Typically, pairs of antibodies (Abs) or antibody fragments (Fabs) that are capable of forming a sandwiching with the target are identified through a slow, guess-and-check method with panels of candidate binding partners. Additionally, sandwich assays that are reliant on commercial antibodies can suffer from changes to reagent quality outside the researchers' control. This report presents a reimagined and simplified phage display selection protocol that directly identifies sandwich binding peptides and Fabs. The approach yielded two sandwich pairs, one peptide-peptide and one Fab-peptide sandwich for the cancer and Parkinson's disease biomarker DJ-1. Requiring just a few weeks to identify, the sandwich pairs delivered apparent affinity that is comparable to other commercial peptide and antibody sandwiches. The results reported here could expand the availability of sandwich binding partners for a wide range of clinical biomarker assays.

Published
2023

2. Single-molecule Taq DNA polymerase dynamics

Author

Turvey, Mackenzie W, Gabriel, Kristin N, Lee, Wonbae, Taulbee, Jeffrey J, Kim, Joshua K, Chen, Silu, Lau, Calvin J, Kattan, Rebecca E, Pham, Jenifer T, Majumdar, Sudipta, Garcia, Davil, Weiss, Gregory A, and Collins, Philip G

Subjects
Generic health relevance, Catalysis, DNA Replication, Kinetics, Nucleotides, Taq Polymerase
Abstract

Taq DNA polymerase functions at elevated temperatures with fast conformational dynamics-regimes previously inaccessible to mechanistic, single-molecule studies. Here, single-walled carbon nanotube transistors recorded the motions of Taq molecules processing matched or mismatched template-deoxynucleotide triphosphate pairs from 22° to 85°C. By using four enzyme orientations, the whole-enzyme closures of nucleotide incorporations were distinguished from more rapid, 20-μs closures of Taq's fingers domain testing complementarity and orientation. On average, one transient closure was observed for every nucleotide binding event; even complementary substrate pairs averaged five transient closures between each catalytic incorporation at 72°C. The rate and duration of the transient closures and the catalytic events had almost no temperature dependence, leaving all of Taq's temperature sensitivity to its rate-determining open state.

Published
2022

3. Reengineering the specificity of the highly selective Clostridium botulinum protease via directed evolution

Author

Dyer, Rebekah P, Isoda, Hariny M, Salcedo, Gabriela S, Speciale, Gaetano, Fletcher, Madison H, Le, Linh Q, Liu, Yi, Brami-Cherrier, Karen, Malik, Shiazah Z, Vazquez-Cintron, Edwin J, Chu, Andrew C, Rupp, David C, Jacky, Birgitte PS, Nguyen, Thu TM, Katz, Benjamin B, Steward, Lance E, Majumdar, Sudipta, Brideau-Andersen, Amy D, and Weiss, Gregory A

Subjects
Biochemistry and Cell Biology, Biological Sciences, Emerging Infectious Diseases, Foodborne Illness, Infectious Diseases, Prevention, Botulinum Toxins, Type A, Catalysis, Catalytic Domain, Clostridium botulinum, Peptide Hydrolases, Protein Engineering, Substrate Specificity
Abstract

The botulinum neurotoxin serotype A (BoNT/A) cuts a single peptide bond in SNAP25, an activity used to treat a wide range of diseases. Reengineering the substrate specificity of BoNT/A's protease domain (LC/A) could expand its therapeutic applications; however, LC/A's extended substrate recognition (≈ 60 residues) challenges conventional approaches. We report a directed evolution method for retargeting LC/A and retaining its exquisite specificity. The resultant eight-mutation LC/A (omLC/A) has improved cleavage specificity and catalytic efficiency (1300- and 120-fold, respectively) for SNAP23 versus SNAP25 compared to a previously reported LC/A variant. Importantly, the BoNT/A holotoxin equipped with omLC/A retains its ability to form full-length holotoxin, infiltrate neurons, and cleave SNAP23. The identification of substrate control loops outside BoNT/A's active site could guide the design of improved BoNT proteases and inhibitors.

Published
2022

4. Predicting COVID-19 Severity with a Specific Nucleocapsid Antibody plus Disease Risk Factor Score

Author

Sen, Sanjana R, Sanders, Emily C, Gabriel, Kristin N, Miller, Brian M, Isoda, Hariny M, Salcedo, Gabriela S, Garrido, Jason E, Dyer, Rebekah P, Nakajima, Rie, Jain, Aarti, Caldaruse, Ana-Maria, Santos, Alicia M, Bhuvan, Keertna, Tifrea, Delia F, Ricks-Oddie, Joni L, Felgner, Philip L, Edwards, Robert A, Majumdar, Sudipta, and Weiss, Gregory A

Subjects
Microbiology, Biological Sciences, Coronaviruses Disparities and At-Risk Populations, Emerging Infectious Diseases, Infectious Diseases, Biotechnology, Prevention, Coronaviruses, 4.1 Discovery and preclinical testing of markers and technologies, Infection, Good Health and Well Being, Antibodies, Viral, COVID-19, Cell Surface Display Techniques, Coronavirus Nucleocapsid Proteins, Enzyme-Linked Immunosorbent Assay, Epitopes, Humans, Nucleocapsid, Phosphoproteins, Prognosis, Risk Factors, SARS-CoV-2, Severity of Illness Index, coronaviruses, epitope mapping, phage display, prognostic, Immunology
Abstract

Effective methods for predicting COVID-19 disease trajectories are urgently needed. Here, enzyme-linked immunosorbent assay (ELISA) and coronavirus antigen microarray (COVAM) analysis mapped antibody epitopes in the plasma of COVID-19 patients (n = 86) experiencing a wide range of disease states. The experiments identified antibodies to a 21-residue epitope from nucleocapsid (termed Ep9) associated with severe disease, including admission to the intensive care unit (ICU), requirement for ventilators, or death. Importantly, anti-Ep9 antibodies can be detected within 6 days post-symptom onset and sometimes within 1 day. Furthermore, anti-Ep9 antibodies correlate with various comorbidities and hallmarks of immune hyperactivity. We introduce a simple-to-calculate, disease risk factor score to quantitate each patient's comorbidities and age. For patients with anti-Ep9 antibodies, scores above 3.0 predict more severe disease outcomes with a 13.42 likelihood ratio (96.7% specificity). The results lay the groundwork for a new type of COVID-19 prognostic to allow early identification and triage of high-risk patients. Such information could guide more effective therapeutic intervention.IMPORTANCE The COVID-19 pandemic has resulted in over two million deaths worldwide. Despite efforts to fight the virus, the disease continues to overwhelm hospitals with severely ill patients. Diagnosis of COVID-19 is readily accomplished through a multitude of reliable testing platforms; however, prognostic prediction remains elusive. To this end, we identified a short epitope from the SARS-CoV-2 nucleocapsid protein and also a disease risk factor score based upon comorbidities and age. The presence of antibodies specifically binding to this epitope plus a score cutoff can predict severe COVID-19 outcomes with 96.7% specificity.

Published
2021

5. Predicting COVID-19 Severity with a Specific Nucleocapsid Antibody plus Disease Risk Factor Score.

Author

Sen, Sanjana R, Sanders, Emily C, Gabriel, Kristin N, Miller, Brian M, Isoda, Hariny M, Salcedo, Gabriela S, Garrido, Jason E, Dyer, Rebekah P, Nakajima, Rie, Jain, Aarti, Caldaruse, Ana-Maria, Santos, Alicia M, Bhuvan, Keertna, Tifrea, Delia F, Ricks-Oddie, Joni L, Felgner, Philip L, Edwards, Robert A, Majumdar, Sudipta, and Weiss, Gregory A

Subjects
Humans, Nucleocapsid, Phosphoproteins, Antibodies, Viral, Epitopes, Enzyme-Linked Immunosorbent Assay, Prognosis, Severity of Illness Index, Risk Factors, Cell Surface Display Techniques, COVID-19, SARS-CoV-2, Coronavirus Nucleocapsid Proteins, coronaviruses, epitope mapping, phage display, prognostic, Biotechnology, Emerging Infectious Diseases, Patient Safety, Prevention, Infectious Diseases, Biodefense, Vaccine Related, 4.1 Discovery and preclinical testing of markers and technologies
Abstract

Effective methods for predicting COVID-19 disease trajectories are urgently needed. Here, enzyme-linked immunosorbent assay (ELISA) and coronavirus antigen microarray (COVAM) analysis mapped antibody epitopes in the plasma of COVID-19 patients (n = 86) experiencing a wide range of disease states. The experiments identified antibodies to a 21-residue epitope from nucleocapsid (termed Ep9) associated with severe disease, including admission to the intensive care unit (ICU), requirement for ventilators, or death. Importantly, anti-Ep9 antibodies can be detected within 6 days post-symptom onset and sometimes within 1 day. Furthermore, anti-Ep9 antibodies correlate with various comorbidities and hallmarks of immune hyperactivity. We introduce a simple-to-calculate, disease risk factor score to quantitate each patient's comorbidities and age. For patients with anti-Ep9 antibodies, scores above 3.0 predict more severe disease outcomes with a 13.42 likelihood ratio (96.7% specificity). The results lay the groundwork for a new type of COVID-19 prognostic to allow early identification and triage of high-risk patients. Such information could guide more effective therapeutic intervention.IMPORTANCE The COVID-19 pandemic has resulted in over two million deaths worldwide. Despite efforts to fight the virus, the disease continues to overwhelm hospitals with severely ill patients. Diagnosis of COVID-19 is readily accomplished through a multitude of reliable testing platforms; however, prognostic prediction remains elusive. To this end, we identified a short epitope from the SARS-CoV-2 nucleocapsid protein and also a disease risk factor score based upon comorbidities and age. The presence of antibodies specifically binding to this epitope plus a score cutoff can predict severe COVID-19 outcomes with 96.7% specificity.

Published
2021

6. Engineering SNAP23 specificity into the highly selective Clostridium botulinum protease

Author

Dyer, Rebekah P, Isoda, Hariny M, Salcedo, Gabriela S, Speciale, Gaetano, Fletcher, Madison H, Le, Linh Q, Liu, Yi, Malik, Shiazah Z, Vazquez-Cintron, Edwin J, Chu, Andrew C, Rupp, David C, Jacky, Birgitte PS, Nguyen, Thu TM, Steward, Lance E, Majumdar, Sudipta, Brideau-Andersen, Amy D, and Weiss, Gregory A

Subjects
BoNT/A, Botulinum neurotoxin, Directed evolution, SNAP23, SNAP25, Pharmacology and Pharmaceutical Sciences, Toxicology
Published
2021

7. Viruses Masquerading as Antibodies in Biosensors: The Development of the Virus BioResistor

Author

Bhasin, Apurva, Drago, Nicholas P, Majumdar, Sudipta, Sanders, Emily C, Weiss, Gregory A, and Penner, Reginald M

Subjects
Analytical Chemistry, Chemical Sciences, Bioengineering, Biotechnology, Antibodies, Bacteriophage M13, Biomarkers, Tumor, Biosensing Techniques, Bridged Bicyclo Compounds, Heterocyclic, Electrodes, Humans, Limit of Detection, Nanowires, Neoplasms, Peptide Library, Polymers, Protein Deglycase DJ-1, Quartz Crystal Microbalance Techniques, Reproducibility of Results, Signal-To-Noise Ratio, General Chemistry, Chemical sciences
Abstract

The 2018 Nobel Prize in Chemistry recognized in vitro evolution, including the development by George Smith and Gregory Winter of phage display, a technology for engineering the functional capabilities of antibodies into viruses. Such bacteriophages solve inherent problems with antibodies, including their high cost, thermal lability, and propensity to aggregate. While phage display accelerated the discovery of peptide and protein motifs for recognition and binding to proteins in a variety of applications, the development of biosensors using intact phage particles was largely unexplored in the early 2000s. Virus particles, 16.5 MDa in size and assembled from thousands of proteins, could not simply be substituted for antibodies in any existing biosensor architectures.Incorporating viruses into biosensors required us to answer several questions: What process will allow the incorporation of viruses into a functional bioaffinity layer? How can the binding of a protein disease marker to a virus particle be electrically transduced to produce a signal? Will the variable salt concentration of a bodily fluid interfere with electrical transduction? A completely new biosensor architecture and a new scheme for electrical transduction of the binding of molecules to viruses were required.This Account describes the highlights of a research program launched in 2006 that answered these questions. These efforts culminated in 2018 in the invention of a biosensor specifically designed to interface with virus particles: the Virus BioResistor (VBR). The VBR is a resistor consisting of a conductive polymer matrix in which M13 virus particles are entrained. The electrical impedance of this resistor, measured across 4 orders of magnitude in frequency, simultaneously measures the concentration of a target protein and the ionic conductivity of the medium in which the resistor is immersed. Large signal amplitudes coupled with the inherent simplicity of the VBR sensor design result in high signal-to-noise ratio (S/N > 100) and excellent sensor-to-sensor reproducibility. Using this new device, we have measured the urinary bladder cancer biomarker nucleic acid deglycase (DJ-1) in urine samples. This optimized VBR is characterized by extremely low sensor-to-sensor coefficients of variation in the range of 3-7% across the DJ-1 binding curve down to a limit of quantitation of 30 pM, encompassing 4 orders of magnitude in concentration.

Published
2020

8. Correction to Virus Bioresistor (VBR) for the Detection of the Bladder Cancer Marker DJ‑1 in Urine at 10 pM in One Minute

Author

Bhasin, Apurva, Sanders, Emily C, Ziegler, Joshua M, Briggs, Jeffrey S, Drago, Nicholas P, Attar, Aisha M, Santos, Alicia M, True, Marie Y, Ogata, Alana F, Yoon, Debora V, Majumdar, Sudipta, Wheat, Andrew J, Patterson, Shae V, Weiss, Gregory A, and Penner, Reginald M

Subjects
Analytical Chemistry, Other Chemical Sciences
Abstract

The author list contained an error: Gregory A. Weiss was not identified as a corresponding author. Both of the corresponding authors, Gregory A. Weiss and Reginald M. Penner, are indicated in this Addition and Correction.

Published
2020

9. 3D-Printed Labware for High-Throughput Immobilization of Enzymes

Author

Spano, Michael B, Tran, Brandan H, Majumdar, Sudipta, and Weiss, Gregory A

Subjects
Biocatalysis, Catalysis, Enzymes, Immobilized, Laccase, Printing, Three-Dimensional, Medicinal and Biomolecular Chemistry, Organic Chemistry
Abstract

In continuous flow biocatalysis, chemical transformations can occur under milder, greener, more scalable, and safer conditions than conventional organic synthesis. However, the method typically involves extensive screening to optimize each enzyme's immobilization on its solid support material. The task of weighing solids for large numbers of experiments poses a bottleneck for screening enzyme immobilization conditions. For example, screening conditions often require multiple replicates exploring different support chemistries, buffer compositions, and temperatures. Thus, we report 3D-printed labware designed to measure and handle solids in multichannel format and expedite screening of enzyme immobilization conditions. To demonstrate the generality of these advances, alkaline phosphatase, glucose dehydrogenase, and laccase were screened for immobilization efficiency on seven resins. The results illustrate the requirements for optimization of each enzyme's loading and resin choice for optimal catalytic performance. Here, 3D-printed labware can decrease the requirements for an experimentalist's time by >95%. The approach to rapid optimization of enzyme immobilization is applicable to any enzyme and many solid support resins. Furthermore, the reported devices deliver precise and accurate aliquots of essentially any granular solid material.

Published
2020

10. Photostable and Proteolysis-Resistant Förster Resonance Energy Transfer-Based Calcium Biosensor

Author

Nguyen, Dat, Behrens, Danielle M, Sen, Sanjana, Najdahmadi, Avid, Pham, Jessica N, Speciale, Gaetano, Lawrence, Micah M, Majumdar, Sudipta, Weiss, Gregory A, and Botvinick, Elliot L

Subjects
Chemical Engineering, Engineering, Bioengineering, Biotechnology, Affordable and Clean Energy, Animals, Batrachoidiformes, Calcium, Fluorescence Resonance Energy Transfer, Photochemical Processes, Proteolysis, Troponin C, Analytical Chemistry, Other Chemical Sciences, Medical biochemistry and metabolomics, Analytical chemistry, Chemical engineering
Abstract

Molecular sensors from protein engineering offer new methods to sensitively bind to and detect target analytes for a wide range of applications. For example, these sensors can be integrated into probes for implantation, and then yield new and valuable physiological information. Here, a new Förster resonance energy transfer (FRET)-based sensor is integrated with an optical fiber to yield a device measuring free Ca2+. This membrane encapsulated optical fiber (MEOF) device is composed of a sensor matrix that fills poly(tetrafluoroethylene) (PTFE) with an engineered troponin C (TnC) protein fused to a pair of FRET fluorophores. The FRET efficiency is modulated upon Ca2+ ion binding. The probe further comprises a second, size-excluding filter membrane that is synthesized by filling the pores of a PTFE matrix with a poly(ethylene glycol) dimethacrylate (PEGDMA) hydrogel; this design ensures protection from circulating proteases and the foreign body response. The two membranes are stacked and placed on a thin, silica optical fiber for optical excitation and detection. Results show the biosensor responds to changes in Ca2+ concentration within minutes with a sensitivity ranging from 0.01 to 10 mM Ca2+, allowing discrimination of hyper- and hypocalcemia. Furthermore, the system reversibly binds Ca2+ to allow continuous monitoring. This work paves the way for the use of engineered structure-switching proteins for continuous optical monitoring in a large number of applications.

Published
2020

11. Photostable and Proteolysis-Resistant Förster Resonance Energy Transfer-Based Calcium Biosensor

Author

Nguyen, Dat, Behrens, Danielle M, Sen, Sanjana, Najdahmadi, Avid, Pham, Jessica N, Speciale, Gaetano, Lawrence, Micah M, Majumdar, Sudipta, Weiss, Gregory A, and Botvinick, Elliot L

Subjects
Chemical Engineering, Engineering, Bioengineering, Affordable and Clean Energy, Animals, Batrachoidiformes, Calcium, Fluorescence Resonance Energy Transfer, Photochemical Processes, Proteolysis, Troponin C, Analytical Chemistry, Other Chemical Sciences, Medical biochemistry and metabolomics, Analytical chemistry, Chemical engineering
Abstract

Molecular sensors from protein engineering offer new methods to sensitively bind to and detect target analytes for a wide range of applications. For example, these sensors can be integrated into probes for implantation, and then yield new and valuable physiological information. Here, a new Förster resonance energy transfer (FRET)-based sensor is integrated with an optical fiber to yield a device measuring free Ca2+. This membrane encapsulated optical fiber (MEOF) device is composed of a sensor matrix that fills poly(tetrafluoroethylene) (PTFE) with an engineered troponin C (TnC) protein fused to a pair of FRET fluorophores. The FRET efficiency is modulated upon Ca2+ ion binding. The probe further comprises a second, size-excluding filter membrane that is synthesized by filling the pores of a PTFE matrix with a poly(ethylene glycol) dimethacrylate (PEGDMA) hydrogel; this design ensures protection from circulating proteases and the foreign body response. The two membranes are stacked and placed on a thin, silica optical fiber for optical excitation and detection. Results show the biosensor responds to changes in Ca2+ concentration within minutes with a sensitivity ranging from 0.01 to 10 mM Ca2+, allowing discrimination of hyper- and hypocalcemia. Furthermore, the system reversibly binds Ca2+ to allow continuous monitoring. This work paves the way for the use of engineered structure-switching proteins for continuous optical monitoring in a large number of applications.

Published
2020

12. Pyrocinchonimides Conjugate to Amine Groups on Proteins via Imide Transfer

Author

Richardson, Mark B, Gabriel, Kristin N, Garcia, Joseph A, Ashby, Shareen N, Dyer, Rebekah P, Kim, Joshua K, Lau, Calvin J, Hong, John, Le Tourneau, Ryan J, Sen, Sanjana, Narel, David L, Katz, Benjamin B, Ziller, Joseph W, Majumdar, Sudipta, Collins, Philip G, and Weiss, Gregory A

Subjects
Organic Chemistry, Chemical Sciences, Generic health relevance, Amines, Hydrogen-Ion Concentration, Imides, Kinetics, Lysine, Proteins, Solvents, Sulfhydryl Compounds, Thermodynamics, Medicinal and Biomolecular Chemistry, Biochemistry and Cell Biology, Biochemistry and cell biology, Medicinal and biomolecular chemistry
Abstract

Advances in bioconjugation, the ability to link biomolecules to each other, small molecules, surfaces, and more, can spur the development of advanced materials and therapeutics. We have discovered that pyrocinchonimide, the dimethylated analogue of maleimide, undergoes a surprising transformation with biomolecules. The reaction targets amines and involves an imide transfer, which has not been previously reported for bioconjugation purposes. Despite their similarity to maleimides, pyrocinchonimides do not react with free thiols. Though both lysine residues and the N-termini of proteins can receive the transferred imide, the reaction also exhibits a marked preference for certain amines that cannot solely be ascribed to solvent accessibility. This property is peculiar among amine-targeting reactions and can reduce combinatorial diversity when many available reactive amines are available, such as in the formation of antibody-drug conjugates. Unlike amides, the modification undergoes very slow reversion under high pH conditions. The reaction offers a thermodynamically controlled route to single or multiple modifications of proteins for a wide range of applications.

Published
2020

13. Pyrocinchonimides Conjugate to Amine Groups on Proteins via Imide Transfer

Author

Richardson, Mark B, Gabriel, Kristin N, Garcia, Joseph A, Ashby, Shareen N, Dyer, Rebekah P, Kim, Joshua K, Lau, Calvin J, Hong, John, Le Tourneau, Ryan J, Sen, Sanjana, Narel, David L, Katz, Benjamin B, Ziller, Joseph W, Majumdar, Sudipta, Collins, Philip G, and Weiss, Gregory A

Subjects
Generic health relevance, Amines, Hydrogen-Ion Concentration, Imides, Kinetics, Lysine, Proteins, Solvents, Sulfhydryl Compounds, Thermodynamics, Medicinal and Biomolecular Chemistry, Organic Chemistry, Biochemistry and Cell Biology
Abstract

Advances in bioconjugation, the ability to link biomolecules to each other, small molecules, surfaces, and more, can spur the development of advanced materials and therapeutics. We have discovered that pyrocinchonimide, the dimethylated analogue of maleimide, undergoes a surprising transformation with biomolecules. The reaction targets amines and involves an imide transfer, which has not been previously reported for bioconjugation purposes. Despite their similarity to maleimides, pyrocinchonimides do not react with free thiols. Though both lysine residues and the N-termini of proteins can receive the transferred imide, the reaction also exhibits a marked preference for certain amines that cannot solely be ascribed to solvent accessibility. This property is peculiar among amine-targeting reactions and can reduce combinatorial diversity when many available reactive amines are available, such as in the formation of antibody-drug conjugates. Unlike amides, the modification undergoes very slow reversion under high pH conditions. The reaction offers a thermodynamically controlled route to single or multiple modifications of proteins for a wide range of applications.

Published
2020

14. Virus Bioresistor (VBR) for Detection of Bladder Cancer Marker DJ‑1 in Urine at 10 pM in One Minute

Author

Bhasin, Apurva, Sanders, Emily C, Ziegler, Joshua M, Briggs, Jeffrey S, Drago, Nicholas P, Attar, Aisha M, Santos, Alicia M, True, Marie Y, Ogata, Alana F, Yoon, Debora V, Majumdar, Sudipta, Wheat, Andrew J, Patterson, Shae V, Weiss, Gregory A, and Penner, Reginald M

Subjects
Analytical Chemistry, Chemical Sciences, Bacteriophage M13, Biomarkers, Tumor, Biosensing Techniques, Humans, Protein Deglycase DJ-1, Time Factors, Urinary Bladder Neoplasms, Other Chemical Sciences, Medical biochemistry and metabolomics, Analytical chemistry, Chemical engineering
Abstract

DJ-1, a 20.7 kDa protein, is overexpressed in people who have bladder cancer (BC). Its elevated concentration in urine allows it to serve as a marker for BC. However, no biosensor for the detection of DJ-1 has been demonstrated. Here, we describe a virus bioresistor (VBR) capable of detecting DJ-1 in urine at a concentration of 10 pM in 1 min. The VBR consists of a pair of millimeter-scale gold electrodes that measure the electrical impedance of an ultrathin (≈ 150-200 nm), two-layer polymeric channel. The top layer of this channel (90-105 nm in thickness) consists of an electrodeposited virus-PEDOT (PEDOT is poly(3,4-ethylenedioxythiophene)) composite containing embedded M13 virus particles that are engineered to recognize and bind to the target protein of interest, DJ-1. The bottom layer consists of spin-coated PEDOT-PSS (poly(styrenesulfonate)). Together, these two layers constitute a current divider. We demonstrate here that reducing the thickness of the bottom PEDOT-PSS layer increases its resistance and concentrates the resistance drop of the channel in the top virus-PEDOT layer, thereby increasing the sensitivity of the VBR and enabling the detection of DJ-1. Large signal amplitudes coupled with the inherent simplicity of the VBR sensor design result in high signal-to-noise (S/N > 100) and excellent sensor-to-sensor reproducibility characterized by coefficients of variation in the range of 3-7% across the DJ-1 binding curve down to a concentration of 30 pM, near the 10 pM limit of detection (LOD), encompassing four orders of magnitude in concentration.

Published
2020

15. Virus Bioresistor (VBR) for Detection of Bladder Cancer Marker DJ‑1 in Urine at 10 pM in One Minute

Author

Bhasin, Apurva, Sanders, Emily C, Ziegler, Joshua M, Briggs, Jeffrey S, Drago, Nicholas P, Attar, Aisha M, Santos, Alicia M, True, Marie Y, Ogata, Alana F, Yoon, Debora V, Majumdar, Sudipta, Wheat, Andrew J, Patterson, Shae V, Weiss, Gregory A, and Penner, Reginald M

Subjects
Bacteriophage M13, Biomarkers, Tumor, Biosensing Techniques, Humans, Protein Deglycase DJ-1, Time Factors, Urinary Bladder Neoplasms, Analytical Chemistry, Other Chemical Sciences
Abstract

DJ-1, a 20.7 kDa protein, is overexpressed in people who have bladder cancer (BC). Its elevated concentration in urine allows it to serve as a marker for BC. However, no biosensor for the detection of DJ-1 has been demonstrated. Here, we describe a virus bioresistor (VBR) capable of detecting DJ-1 in urine at a concentration of 10 pM in 1 min. The VBR consists of a pair of millimeter-scale gold electrodes that measure the electrical impedance of an ultrathin (≈ 150-200 nm), two-layer polymeric channel. The top layer of this channel (90-105 nm in thickness) consists of an electrodeposited virus-PEDOT (PEDOT is poly(3,4-ethylenedioxythiophene)) composite containing embedded M13 virus particles that are engineered to recognize and bind to the target protein of interest, DJ-1. The bottom layer consists of spin-coated PEDOT-PSS (poly(styrenesulfonate)). Together, these two layers constitute a current divider. We demonstrate here that reducing the thickness of the bottom PEDOT-PSS layer increases its resistance and concentrates the resistance drop of the channel in the top virus-PEDOT layer, thereby increasing the sensitivity of the VBR and enabling the detection of DJ-1. Large signal amplitudes coupled with the inherent simplicity of the VBR sensor design result in high signal-to-noise (S/N > 100) and excellent sensor-to-sensor reproducibility characterized by coefficients of variation in the range of 3-7% across the DJ-1 binding curve down to a concentration of 30 pM, near the 10 pM limit of detection (LOD), encompassing four orders of magnitude in concentration.

Published
2020

16. Vortex fluidics-mediated DNA rescue from formalin-fixed museum specimens.

Author

Totoiu, Christian A, Phillips, Jessica M, Reese, Aspen T, Majumdar, Sudipta, Girguis, Peter R, Raston, Colin L, and Weiss, Gregory A

Subjects
Animals, Nephropidae, Formaldehyde, DNA, Tissue Fixation, Polymerase Chain Reaction, Base Sequence, Museums, Hydrodynamics, General Science & Technology
Abstract

DNA from formalin-preserved tissue could unlock a vast repository of genetic information stored in museums worldwide. However, formaldehyde crosslinks proteins and DNA, and prevents ready amplification and DNA sequencing. Formaldehyde acylation also fragments the DNA. Treatment with proteinase K proteolyzes crosslinked proteins to rescue the DNA, though the process is quite slow. To reduce processing time and improve rescue efficiency, we applied the mechanical energy of a vortex fluidic device (VFD) to drive the catalytic activity of proteinase K and recover DNA from American lobster tissue (Homarus americanus) fixed in 3.7% formalin for >1-year. A scan of VFD rotational speeds identified the optimal rotational speed for recovery of PCR-amplifiable DNA and while 500+ base pairs were sequenced, shorter read lengths were more consistently obtained. This VFD-based method also effectively recovered DNA from formalin-preserved samples. The results provide a roadmap for exploring DNA from millions of historical and even extinct species.

Published
2020

17. Vortex fluidics-mediated DNA rescue from formalin-fixed museum specimens

Author

Totoiu, Christian A, Phillips, Jessica M, Reese, Aspen T, Majumdar, Sudipta, Girguis, Peter R, Raston, Colin L, and Weiss, Gregory A

Subjects
Biological Sciences, Genetics, Animals, Base Sequence, DNA, Formaldehyde, Hydrodynamics, Museums, Nephropidae, Polymerase Chain Reaction, Tissue Fixation, General Science & Technology
Abstract

DNA from formalin-preserved tissue could unlock a vast repository of genetic information stored in museums worldwide. However, formaldehyde crosslinks proteins and DNA, and prevents ready amplification and DNA sequencing. Formaldehyde acylation also fragments the DNA. Treatment with proteinase K proteolyzes crosslinked proteins to rescue the DNA, though the process is quite slow. To reduce processing time and improve rescue efficiency, we applied the mechanical energy of a vortex fluidic device (VFD) to drive the catalytic activity of proteinase K and recover DNA from American lobster tissue (Homarus americanus) fixed in 3.7% formalin for >1-year. A scan of VFD rotational speeds identified the optimal rotational speed for recovery of PCR-amplifiable DNA and while 500+ base pairs were sequenced, shorter read lengths were more consistently obtained. This VFD-based method also effectively recovered DNA from formalin-preserved samples. The results provide a roadmap for exploring DNA from millions of historical and even extinct species.

Published
2020

18. Electrochemical Quantification of Glycated and Non-glycated Human Serum Albumin in Synthetic Urine

Author

Attar, Aisha M, Richardson, Mark B, Speciale, Gaetano, Majumdar, Sudipta, Dyer, Rebekah P, Sanders, Emily C, Penner, Reginald M, and Weiss, Gregory A

Subjects
Analytical Chemistry, Engineering, Chemical Sciences, Diabetes, Biosensing Techniques, Electrochemical Techniques, Enzymes, Immobilized, Equipment Design, Glycation End Products, Advanced, Humans, Models, Biological, Serum Albumin, Serum Albumin, Human, Tetrahydrofolate Dehydrogenase, Glycated Serum Albumin, human serum albumin, glycated albumin, polythiophene, iminodiacetic acid, boronic acid, dihydrofolate reductase, biosensor, Nanoscience & Nanotechnology, Chemical sciences, Physical sciences
Abstract

A polymer-based electrode capable of specific detection of human serum albumin, and its glycated derivatives, is described. The sensor is constructed from a glass microscope slide coated with a synthesized, polythiophene film bearing a protected, iminodiacetic acid motif. The electrode surface is then further elaborated to a functional biosensor through deprotection of the iminodiacetic acid, followed by metal-affinity immobilization of a specific and high-affinity, albumin ligand. Albumin was then quantified in buffer and synthetic urine via electrochemical impedance spectroscopy. Glycated albumin was next bound to a boronic acid-modified, single-cysteine dihydrofolate reductase variant to quantify glycation ratios by square-wave voltammetry. The platform offers high sensitivity, specificity, and reproducibility in an inexpensive arrangement. The detection limits exceed the requirements for intermediate-term glycemic control monitoring in diabetes patients at 5 and 1 nM for albumin and its glycated forms, respectively.

Published
2019

19. Electrochemical Quantification of Glycated and Non-glycated Human Serum Albumin in Synthetic Urine

Author

Attar, Aisha M, Richardson, Mark B, Speciale, Gaetano, Majumdar, Sudipta, Dyer, Rebekah P, Sanders, Emily C, Penner, Reginald M, and Weiss, Gregory A

Subjects
Diabetes, Biosensing Techniques, Electrochemical Techniques, Enzymes, Immobilized, Equipment Design, Glycation End Products, Advanced, Humans, Models, Biological, Serum Albumin, Serum Albumin, Human, Tetrahydrofolate Dehydrogenase, Glycated Serum Albumin, human serum albumin, glycated albumin, polythiophene, iminodiacetic acid, boronic acid, dihydrofolate reductase, biosensor, Chemical Sciences, Engineering, Nanoscience & Nanotechnology
Abstract

A polymer-based electrode capable of specific detection of human serum albumin, and its glycated derivatives, is described. The sensor is constructed from a glass microscope slide coated with a synthesized, polythiophene film bearing a protected, iminodiacetic acid motif. The electrode surface is then further elaborated to a functional biosensor through deprotection of the iminodiacetic acid, followed by metal-affinity immobilization of a specific and high-affinity, albumin ligand. Albumin was then quantified in buffer and synthetic urine via electrochemical impedance spectroscopy. Glycated albumin was next bound to a boronic acid-modified, single-cysteine dihydrofolate reductase variant to quantify glycation ratios by square-wave voltammetry. The platform offers high sensitivity, specificity, and reproducibility in an inexpensive arrangement. The detection limits exceed the requirements for intermediate-term glycemic control monitoring in diabetes patients at 5 and 1 nM for albumin and its glycated forms, respectively.

Published
2019

20. Directed evolution and biophysical characterization of a full-length, soluble, human caveolin-1 variant

Author

Smith, Joshua N, Edgar, Joshua M, Balk, J Mark, Iftikhar, Mariam, Fong, Jessica C, Olsen, Tivoli J, Fishman, Dmitry A, Majumdar, Sudipta, and Weiss, Gregory A

Subjects
Biochemistry and Cell Biology, Biological Sciences, Biotechnology, 1.1 Normal biological development and functioning, Underpinning research, Catalytic Domain, Caveolin 1, Cells, Cultured, Cyclic AMP-Dependent Protein Kinases, Directed Molecular Evolution, Escherichia coli, HIV Envelope Protein gp41, Humans, Peptide Library, Protein Domains, Protein Engineering, Protein Folding, RNA-Binding Proteins, Signal Transduction, Thermodynamics, Phage display, Membrane proteins, Caveolin, Caveolae, Oligomerization, Biophysics, Biochemistry & Molecular Biology, Biological sciences
Abstract

Protein engineering by directed evolution can alter proteins' structures, properties, and functions. However, membrane proteins, despite their importance to living organisms, remain relatively unexplored as targets for protein engineering and directed evolution. This gap in capabilities likely results from the tendency of membrane proteins to aggregate and fail to overexpress in bacteria cells. For example, the membrane protein caveolin-1 has been implicated in many cell signaling pathways and diseases, yet the full-length protein is too aggregation-prone for detailed mutagenesis, directed evolution, and biophysical characterization. Using a phage-displayed library of full-length caveolin-1 variants, directed evolution with alternating subtractive and functional selections isolated a full-length, soluble variant, termed cavsol, for expression in E. coli. Cavsol folds correctly and binds to its known protein ligands HIV gp41, the catalytic domain of cAMP-dependent protein kinase A, and the polymerase I and transcript release factor. As expected, cavsol does not bind off-target proteins. Cellular studies show that cavsol retains the parent protein's ability to localize at the cellular membrane. Unlike truncated versions of caveolin, cavsol forms large, oligomeric complexes consisting of approximately >50 monomeric units without requiring additional cellular components. Cavsol's secondary structure is a mixture of α-helices and β-strands. Isothermal titration calorimetry experiments reveal that cavsol binds to gp41 and PKA with low micromolar binding affinity (KD). In addition to the insights into caveolin structure and function, the approach applied here could be generalized to other membrane proteins.

Published
2018

21. Directed evolution and biophysical characterization of a full-length, soluble, human caveolin-1 variant.

Author

Smith, Joshua N, Edgar, Joshua M, Balk, J Mark, Iftikhar, Mariam, Fong, Jessica C, Olsen, Tivoli J, Fishman, Dmitry A, Majumdar, Sudipta, and Weiss, Gregory A

Subjects
Cells, Cultured, Humans, Escherichia coli, Cyclic AMP-Dependent Protein Kinases, Peptide Library, RNA-Binding Proteins, HIV Envelope Protein gp41, Directed Molecular Evolution, Protein Engineering, Signal Transduction, Catalytic Domain, Protein Folding, Thermodynamics, Caveolin 1, Protein Domains, Biophysics, Caveolae, Caveolin, Membrane proteins, Oligomerization, Phage display, Biotechnology, 1.1 Normal biological development and functioning, Underpinning research, Biological Sciences, Biochemistry & Molecular Biology
Abstract

Protein engineering by directed evolution can alter proteins' structures, properties, and functions. However, membrane proteins, despite their importance to living organisms, remain relatively unexplored as targets for protein engineering and directed evolution. This gap in capabilities likely results from the tendency of membrane proteins to aggregate and fail to overexpress in bacteria cells. For example, the membrane protein caveolin-1 has been implicated in many cell signaling pathways and diseases, yet the full-length protein is too aggregation-prone for detailed mutagenesis, directed evolution, and biophysical characterization. Using a phage-displayed library of full-length caveolin-1 variants, directed evolution with alternating subtractive and functional selections isolated a full-length, soluble variant, termed cavsol, for expression in E. coli. Cavsol folds correctly and binds to its known protein ligands HIV gp41, the catalytic domain of cAMP-dependent protein kinase A, and the polymerase I and transcript release factor. As expected, cavsol does not bind off-target proteins. Cellular studies show that cavsol retains the parent protein's ability to localize at the cellular membrane. Unlike truncated versions of caveolin, cavsol forms large, oligomeric complexes consisting of approximately >50 monomeric units without requiring additional cellular components. Cavsol's secondary structure is a mixture of α-helices and β-strands. Isothermal titration calorimetry experiments reveal that cavsol binds to gp41 and PKA with low micromolar binding affinity (KD). In addition to the insights into caveolin structure and function, the approach applied here could be generalized to other membrane proteins.

Published
2018

22. Continuous flow biocatalysis

Author

Britton, Joshua, Majumdar, Sudipta, and Weiss, Gregory A

Subjects
Engineering, Chemical Sciences, 1.3 Chemical and physical sciences, Underpinning research, Biocatalysis, Bioreactors, Cells, Immobilized, Enzyme Activation, Enzymes, Immobilized, Humans, Pharmaceutical Preparations, Physical Phenomena, Pressure, Surface Properties, Technology, Pharmaceutical, Temperature, General Chemistry, Chemical sciences
Abstract

The continuous flow synthesis of active pharmaceutical ingredients, value-added chemicals, and materials has grown tremendously over the past ten years. This revolution in chemical manufacturing has resulted from innovations in both new methodology and technology. This field, however, has been predominantly focused on synthetic organic chemistry, and the use of biocatalysts in continuous flow systems is only now becoming popular. Although immobilized enzymes and whole cells in batch systems are common, their continuous flow counterparts have grown rapidly over the past two years. With continuous flow systems offering improved mixing, mass transfer, thermal control, pressurized processing, decreased variation, automation, process analytical technology, and in-line purification, the combination of biocatalysis and flow chemistry opens powerful new process windows. This Review explores continuous flow biocatalysts with emphasis on new technology, enzymes, whole cells, co-factor recycling, and immobilization methods for the synthesis of pharmaceuticals, value-added chemicals, and materials.

Published
2018

23. Continuous flow biocatalysis

Author

Britton, Joshua, Majumdar, Sudipta, and Weiss, Gregory A

Subjects
1.3 Chemical and physical sciences, Underpinning research, Biocatalysis, Bioreactors, Cells, Immobilized, Enzyme Activation, Enzymes, Immobilized, Humans, Pharmaceutical Preparations, Physical Phenomena, Pressure, Surface Properties, Technology, Pharmaceutical, Temperature, Chemical Sciences, General Chemistry
Abstract

The continuous flow synthesis of active pharmaceutical ingredients, value-added chemicals, and materials has grown tremendously over the past ten years. This revolution in chemical manufacturing has resulted from innovations in both new methodology and technology. This field, however, has been predominantly focused on synthetic organic chemistry, and the use of biocatalysts in continuous flow systems is only now becoming popular. Although immobilized enzymes and whole cells in batch systems are common, their continuous flow counterparts have grown rapidly over the past two years. With continuous flow systems offering improved mixing, mass transfer, thermal control, pressurized processing, decreased variation, automation, process analytical technology, and in-line purification, the combination of biocatalysis and flow chemistry opens powerful new process windows. This Review explores continuous flow biocatalysts with emphasis on new technology, enzymes, whole cells, co-factor recycling, and immobilization methods for the synthesis of pharmaceuticals, value-added chemicals, and materials.

Published
2018

24. Dimethylmaleimide: a new reagent for protein bioconjugation

Author

Dyer, Rebekah, Richardson, Mark, Garcia, Joseph, Chu, Andrew, Majumdar, Sudipta, and Weiss, Gregory A

Subjects
Rare Diseases, Cancer, Generic health relevance, Good Health and Well Being, Biochemistry and Cell Biology, Physiology, Medical Physiology, Biochemistry & Molecular Biology
Published
2018

25. Dissecting binding of a β-barrel membrane protein by phage display

Author

Meneghini, Luz M, Tripathi, Sarvind, Woodworth, Marcus A, Majumdar, Sudipta, Poulos, Thomas L, and Weiss, Gregory A

Subjects
Biochemistry and Cell Biology, Biological Sciences, Biotechnology, Genetics, Generic health relevance, Amino Acid Sequence, Bacterial Outer Membrane Proteins, Bacteriophage M13, Binding Sites, Capsid Proteins, Cell Surface Display Techniques, Cloning, Molecular, Escherichia coli, Gene Expression, Genetic Vectors, Heme, Hemoglobins, Histidine, Models, Molecular, Protein Binding, Protein Conformation, beta-Strand, Protein Interaction Domains and Motifs, Protein Structure, Tertiary, Recombinant Fusion Proteins, Shigella dysenteriae, Biochemistry and cell biology, Bioinformatics and computational biology, Medical biochemistry and metabolomics
Abstract

Membrane proteins (MPs) constitute a third of all proteomes, and contribute to a myriad of cellular functions including intercellular communication, nutrient transport and energy generation. For example, TonB-dependent transporters (TBDTs) in the outer membrane of Gram-negative bacteria play an essential role transporting iron and other nutrients into the bacterial cell. The inherently hydrophobic surfaces of MPs complicates protein expression, purification, and characterization. Thus, dissecting the functional contributions of individual amino acids or structural features through mutagenesis can be a challenging ordeal. Here, we apply a new approach for the expedited protein characterization of the TBDT ShuA from Shigella dysenteriae, and elucidate the protein's initial steps during heme-uptake. ShuA variants were displayed on the surface of an M13 bacteriophage as fusions to the P8 coat protein. Each ShuA variant was analyzed for its ability to display on the bacteriophage surface, and functionally bind to hemoglobin. This technique streamlines isolation of stable MP variants for rapid characterization of binding to various ligands. Site-directed mutagenesis studies targeting each extracellular loop region of ShuA demonstrate no specific extracellular loop is required for hemoglobin binding. Instead two residues, His420 and His86 mediate this interaction. The results identify a loop susceptible to antibody binding, and also a small molecule motif capable of disrupting ShuA from S. dysenteriae. The approach is generalizable to the dissection of other phage-displayed TBDTs and MPs.

Published
2017

26. Dissecting binding of a β-barrel membrane protein by phage display.

Author

Meneghini, Luz M, Tripathi, Sarvind, Woodworth, Marcus A, Majumdar, Sudipta, Poulos, Thomas L, and Weiss, Gregory A

Subjects
Escherichia coli, Shigella dysenteriae, Bacteriophage M13, Heme, Histidine, Bacterial Outer Membrane Proteins, Hemoglobins, Recombinant Fusion Proteins, Capsid Proteins, Cloning, Molecular, Gene Expression, Binding Sites, Amino Acid Sequence, Protein Structure, Tertiary, Protein Binding, Genetic Vectors, Models, Molecular, Protein Interaction Domains and Motifs, Cell Surface Display Techniques, Protein Conformation, beta-Strand, Biotechnology, Genetics, Generic Health Relevance, Cloning, Molecular, Protein Structure, Tertiary, Models, Protein Conformation, beta-Strand, Biochemistry & Molecular Biology, Biochemistry and Cell Biology
Abstract

Membrane proteins (MPs) constitute a third of all proteomes, and contribute to a myriad of cellular functions including intercellular communication, nutrient transport and energy generation. For example, TonB-dependent transporters (TBDTs) in the outer membrane of Gram-negative bacteria play an essential role transporting iron and other nutrients into the bacterial cell. The inherently hydrophobic surfaces of MPs complicates protein expression, purification, and characterization. Thus, dissecting the functional contributions of individual amino acids or structural features through mutagenesis can be a challenging ordeal. Here, we apply a new approach for the expedited protein characterization of the TBDT ShuA from Shigella dysenteriae, and elucidate the protein's initial steps during heme-uptake. ShuA variants were displayed on the surface of an M13 bacteriophage as fusions to the P8 coat protein. Each ShuA variant was analyzed for its ability to display on the bacteriophage surface, and functionally bind to hemoglobin. This technique streamlines isolation of stable MP variants for rapid characterization of binding to various ligands. Site-directed mutagenesis studies targeting each extracellular loop region of ShuA demonstrate no specific extracellular loop is required for hemoglobin binding. Instead two residues, His420 and His86 mediate this interaction. The results identify a loop susceptible to antibody binding, and also a small molecule motif capable of disrupting ShuA from S. dysenteriae. The approach is generalizable to the dissection of other phage-displayed TBDTs and MPs.

Published
2017

29. Ten‐Minute Protein Purification and Surface Tethering for Continuous‐Flow Biocatalysis

Author

Britton, Joshua, Dyer, Rebekah P, Majumdar, Sudipta, Raston, Colin L, and Weiss, Gregory A

Subjects
Biocatalysis, Chromatography, Affinity, Equipment Design, Escherichia coli, Escherichia coli Proteins, Immobilized Proteins, Isomerases, Luminescent Proteins, Metals, Models, Molecular, Proteins, Time Factors, Tobacco, biocatalysis, continuous flow, multi-step transformations, protein purification, thin films, Chemical Sciences, Organic Chemistry
Abstract

Nature applies enzymatic assembly lines to synthesize bioactive compounds. Inspired by such capabilities, we have developed a facile method for spatially segregating attached enzymes in a continuous-flow, vortex fluidic device (VFD). Fused Hisn -tags at the protein termini allow rapid bioconjugation and consequent purification through complexation with immobilized metal affinity chromatography (IMAC) resin. Six proteins were purified from complex cell lysates to average homogeneities of 76 %. The most challenging to purify, tobacco epi-aristolochene synthase, was purified in only ten minutes from cell lysate to near homogeneity (>90 %). Furthermore, this "reaction-ready" system demonstrated excellent stability during five days of continuous-flow processing. Towards multi-step transformations in continuous flow, proteins were arrayed as ordered zones on the reactor surface allowing segregation of catalysts. Ordering enzymes into zones opens up new opportunities for continuous-flow biosynthesis.

Published
2017

33. Ten‐Minute Protein Purification and Surface Tethering for Continuous‐Flow Biocatalysis

Author

Britton, Joshua, Dyer, Rebekah P, Majumdar, Sudipta, Raston, Colin L, and Weiss, Gregory A

Subjects
Biochemistry and Cell Biology, Biological Sciences, Rare Diseases, Chemical Sciences, Organic Chemistry, Chemical sciences
Abstract

Abstract: Nature applies enzymatic assembly lines to synthesize bioactive compounds. Inspired by such capabilities, we have developed a facile method for spatially segregating attached enzymes in a continuous‐flow, vortex fluidic device (VFD). Fused Hisn‐tags at the protein termini allow rapid bioconjugation and consequent purification through complexation with immobilized metal affinity chromatography (IMAC) resin. Six proteins were purified from complex cell lysates to average homogeneities of 76 %. The most challenging to purify, tobacco epi‐aristolochene synthase, was purified in only ten minutes from cell lysate to near homogeneity (>90 %). Furthermore, this “reaction‐ready” system demonstrated excellent stability during five days of continuous‐flow processing. Towards multi‐step transformations in continuous flow, proteins were arrayed as ordered zones on the reactor surface allowing segregation of catalysts. Ordering enzymes into zones opens up new opportunities for continuous‐flow biosynthesis.

Published
2017

34. Ten-Minute Protein Purification and Surface Tethering for Continuous-Flow Biocatalysis.

Author

Britton, Joshua, Dyer, Rebekah P, Majumdar, Sudipta, Raston, Colin L, and Weiss, Gregory A

Subjects
Escherichia coli, Tobacco, Metals, Isomerases, Proteins, Escherichia coli Proteins, Luminescent Proteins, Chromatography, Affinity, Equipment Design, Models, Molecular, Time Factors, Biocatalysis, Immobilized Proteins, biocatalysis, continuous flow, multi-step transformations, protein purification, thin films, Chromatography, Affinity, Models, Molecular, Chemical Sciences, Organic Chemistry
Abstract

Nature applies enzymatic assembly lines to synthesize bioactive compounds. Inspired by such capabilities, we have developed a facile method for spatially segregating attached enzymes in a continuous-flow, vortex fluidic device (VFD). Fused Hisn -tags at the protein termini allow rapid bioconjugation and consequent purification through complexation with immobilized metal affinity chromatography (IMAC) resin. Six proteins were purified from complex cell lysates to average homogeneities of 76 %. The most challenging to purify, tobacco epi-aristolochene synthase, was purified in only ten minutes from cell lysate to near homogeneity (>90 %). Furthermore, this "reaction-ready" system demonstrated excellent stability during five days of continuous-flow processing. Towards multi-step transformations in continuous flow, proteins were arrayed as ordered zones on the reactor surface allowing segregation of catalysts. Ordering enzymes into zones opens up new opportunities for continuous-flow biosynthesis.

Published
2017

35. Virus-Enabled Biosensor for Human Serum Albumin

Author

Ogata, Alana F, Edgar, Joshua M, Majumdar, Sudipta, Briggs, Jeffrey S, Patterson, Shae V, Tan, Ming X, Kudlacek, Stephan T, Schneider, Christine A, Weiss, Gregory A, and Penner, Reginald M

Subjects
Biotechnology, Bioengineering, Bacteriophage M13, Biosensing Techniques, Bridged Bicyclo Compounds, Heterocyclic, Electric Conductivity, Electric Impedance, Electrodes, Equipment Design, Humans, Limit of Detection, Polymers, Reproducibility of Results, Serum Albumin, Human, Virion, Analytical Chemistry, Other Chemical Sciences
Abstract

The label-free detection of human serum albumin (HSA) in aqueous buffer is demonstrated using a simple, monolithic, two-electrode electrochemical biosensor. In this device, both millimeter-scale electrodes are coated with a thin layer of a composite containing M13 virus particles and the electronically conductive polymer poly(3,4-ethylenedioxy thiophene) or PEDOT. These virus particles, engineered to selectively bind HSA, serve as receptors in this biosensor. The resistance component of the electrical impedance, Zre, measured between these two electrodes provides electrical transduction of HSA binding to the virus-PEDOT film. The analysis of sample volumes as small as 50 μL is made possible using a microfluidic cell. Upon exposure to HSA, virus-PEDOT films show a prompt increase in Zre within 5 s and a stable Zre signal within 15 min. HSA concentrations in the range from 100 nM to 5 μM are detectable. Sensor-to-sensor reproducibility of the HSA measurement is characterized by a coefficient-of-variance (COV) ranging from 2% to 8% across this entire concentration range. In addition, virus-PEDOT sensors successfully detected HSA in synthetic urine solutions.

Published
2017

36. Virus-Enabled Biosensor for Human Serum Albumin.

Author

Ogata, Alana F, Edgar, Joshua M, Majumdar, Sudipta, Briggs, Jeffrey S, Patterson, Shae V, Tan, Ming X, Kudlacek, Stephan T, Schneider, Christine A, Weiss, Gregory A, and Penner, Reginald M

Subjects
Humans, Bacteriophage M13, Virion, Polymers, Reproducibility of Results, Equipment Design, Biosensing Techniques, Electrodes, Electric Conductivity, Electric Impedance, Limit of Detection, Bridged Bicyclo Compounds, Heterocyclic, Serum Albumin, Human, Bridged Bicyclo Compounds, Heterocyclic, Serum Albumin, Human, Bioengineering, Biotechnology, Analytical Chemistry, Chemical Engineering, Other Chemical Sciences
Abstract

The label-free detection of human serum albumin (HSA) in aqueous buffer is demonstrated using a simple, monolithic, two-electrode electrochemical biosensor. In this device, both millimeter-scale electrodes are coated with a thin layer of a composite containing M13 virus particles and the electronically conductive polymer poly(3,4-ethylenedioxy thiophene) or PEDOT. These virus particles, engineered to selectively bind HSA, serve as receptors in this biosensor. The resistance component of the electrical impedance, Zre, measured between these two electrodes provides electrical transduction of HSA binding to the virus-PEDOT film. The analysis of sample volumes as small as 50 μL is made possible using a microfluidic cell. Upon exposure to HSA, virus-PEDOT films show a prompt increase in Zre within 5 s and a stable Zre signal within 15 min. HSA concentrations in the range from 100 nM to 5 μM are detectable. Sensor-to-sensor reproducibility of the HSA measurement is characterized by a coefficient-of-variance (COV) ranging from 2% to 8% across this entire concentration range. In addition, virus-PEDOT sensors successfully detected HSA in synthetic urine solutions.

Published
2017

37. Affinity-Guided Design of Caveolin‑1 Ligands for Deoligomerization

Author

Gilliam, Amanda JH, Smith, Joshua N, Flather, Dylan, Johnston, Kevin M, Gansmiller, Andrew M, Fishman, Dmitry A, Edgar, Joshua M, Balk, Mark, Majumdar, Sudipta, and Weiss, Gregory A

Subjects
Medicinal and Biomolecular Chemistry, Chemical Sciences, Biopolymers, Caveolin 1, Ligands, Organic Chemistry, Pharmacology and Pharmaceutical Sciences, Medicinal & Biomolecular Chemistry, Pharmacology and pharmaceutical sciences, Medicinal and biomolecular chemistry, Organic chemistry
Abstract

Caveolin-1 is a target for academic and pharmaceutical research due to its many cellular roles and associated diseases. We report peptide WL47 (1), a small, high-affinity, selective disrupter of caveolin-1 oligomers. Developed and optimized through screening and analysis of synthetic peptide libraries, ligand 1 has 7500-fold improved affinity compared to its T20 parent ligand and an 80% decrease in sequence length. Ligand 1 will permit targeted study of caveolin-1 function.

Published
2016

38. Affinity-Guided Design of Caveolin-1 Ligands for Deoligomerization.

Author

Gilliam, Amanda JH, Smith, Joshua N, Flather, Dylan, Johnston, Kevin M, Gansmiller, Andrew M, Fishman, Dmitry A, Edgar, Joshua M, Balk, Mark, Majumdar, Sudipta, and Weiss, Gregory A

Subjects
Biopolymers, Ligands, Caveolin 1, Medicinal & Biomolecular Chemistry, Medicinal and Biomolecular Chemistry, Pharmacology and Pharmaceutical Sciences, Organic Chemistry
Abstract

Caveolin-1 is a target for academic and pharmaceutical research due to its many cellular roles and associated diseases. We report peptide WL47 (1), a small, high-affinity, selective disrupter of caveolin-1 oligomers. Developed and optimized through screening and analysis of synthetic peptide libraries, ligand 1 has 7500-fold improved affinity compared to its T20 parent ligand and an 80% decrease in sequence length. Ligand 1 will permit targeted study of caveolin-1 function.

Published
2016

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