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Award Abstract # 1610516
Transient Induced Molecular Electronic Spectroscopy (TIMES) for study of protein-ligand interactions
| NSF Org: |
ECCS Div Of Electrical, Commun & Cyber Sys |
| Awardee: |
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| Initial Amendment Date: | June 3, 2016 |
| Latest Amendment Date: | June 3, 2016 |
| Award Number: | 1610516 |
| Award Instrument: | Standard Grant |
| Program Manager: |
Shubhra Gangopadhyay
ECCS Div Of Electrical, Commun & Cyber Sys ENG Directorate For Engineering |
| Start Date: | June 1, 2016 |
| End Date: | March 31, 2020 (Estimated) |
| Total Intended Award Amount: | $395,197.00 |
| Total Awarded Amount to Date: | $395,197.00 |
| Funds Obligated to Date: |
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| History of Investigator: |
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| Awardee Sponsored Research Office: |
Office of Contract & Grant Admin La Jolla CA US 92093-0934 (858)534-4896 |
| Sponsor Congressional District: |
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| Primary Place of Performance: |
CA US 92093-0407 |
| Primary Place of Performance Congressional District: |
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| Unique Entity Identifier (UEI): |
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| Parent UEI: |
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| NSF Program(s): | CCSS-Comms Circuits & Sens Sys |
| Primary Program Source: |
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| Program Reference Code(s): |
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| Program Element Code(s): |
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| Award Agency Code: | 4900 |
| Fund Agency Code: | 4900 |
| Assistance Listing Number(s): | 47.041 |
ABSTRACT
Title:
Transient Induced Molecular Electronic Spectroscopy (TIMES) for study of protein-ligand interactions
Project Goal:
To test protein-ligand interactions, the key mechanisms for most drugs, without any external disturbances caused by molecular labelling or immobilization.
Nontechnical Abstract:
Protein ligand interaction is one of the most fundamental and widely studied areas in biology and chemistry because of their close relation to many diseases and disease therapies. Nearly all diseases including cancer, neural disorders, infectious diseases, cardiovascular diseases, renal diseases, metabolic diseases, immune diseases, etc. are connected to the abnormality of protein-protein or protein-ligand interactions. Unfortunately, all the current methods for in-vitro protein-ligand tests use either labels (often fluorescent) or ligand immobilization, both of which can produce substantial disruptions and introduce artifacts. These limitations have caused significant delay and cost increase in drug development. A new method is proposed and investigated to fundamentally solve the above problems, allowing precise in-vitro tests of the binding strength and kinetics of proteins ligand interactions to accelerate the process of drug discovery. The work can have significant impact on public health and the country's healthcare by shortening the time and saving the cost for drug discovery. The proposed research will also contribute to education and training of new generation of scientists for multi-disciplinary research involving biology, biochemistry, biophysics and engineering. The research also includes significant outreach activities to engage middle and high school students and underrepresented minority students to advance the STEM efforts.
Technical Abstract:
Since a protein and ligand have a large molecular weight and size difference (e.g.,100 kDa versus 1 kDa), linking organic fluorescent molecules to a protein or ligand can perturb or even change the binding properties. Similarly, the bioactivity of protein depends on its 3D configuration. Immobilization of the molecules limits its degree of freedom for binding, thus often yielding results different from reactions in physiological conditions. Lacking a precise method of in-vitro detection of protein-ligand interactions without any external disturbances has presented a major challenge for mid to late stage drug tests. Drug companies have often conducted unnecessary and unsuccessful human trials while the failures should have been detected earlier if a precise in-vitro test method exists. The most significant scientific and technological contributions of the proposed research will be the development of the method of Transient Induced Electronic Molecular Spectroscopy (TIMES) that allows label-free and immobilization-free detection of protein-ligand interactions. The TIMES method measures the signal caused by the dipole moment change when protein and ligand form protein-ligand complex. When integrated with ultralow noise electronics and microfluidics, the new µTIMES system will enable researchers to collect unprecedented rich information with high timing resolution and enhanced signal-to-noise ratio. This method will be applied to quantitative studies of protein-ligand and protein-aptamer interactions by measuring the dissociation constant and reaction kinetics.
PUBLICATIONS PRODUCED AS A RESULT OF THIS RESEARCH
Note:
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Chung-Lun Hsu, Tiantian Zhang, Yu-Hwa Lo, and Drew A. Hall
"A Low-Noise Gain-Enhanced Readout Amplifier for Induced Molecular Electronic Signal"
Biomedical Circuits and Systems Conference (BioCAS)
, 2015
Tiantian Zhang, Tao Wei, Yuanyuan Han, Heng Ma, Mohammadreza Samieegohar, Ping-Wei Chen, Ian Lian, Yu-Hwa Lo
"Protein-Ligand Interaction Detection with a Novel Method of Transient Induced Molecular Electronic Spectroscopy(TIMES):Experimental and Theoretical Studies"
ACS Central Science
, 2016
10.1021/acscentsci.6b00217
Tiantian Zhang, Ti-Hsuan Ku, Yuanyuan Han, Ramkumar Subramanian, Iftikhar Ahmad Niaz, Hua Luo, Derrick Chang, Jian-Jang Huang, Yu-Hwa Lo
"Transient Induced Molecular Electronic Spectroscopy (TIMES) for study of protein-ligand interactions"
Scientific Reports
, 2016
10.1038/srep35570
Da Ying, Ping-Wei Chen, Chi Tseng, Yu-Hwa Lo, and Drew A. Hall
"A Sub-pA Current Sensing Front-End for Transient Induced Molecular Spectroscopy"
IEEE Symp. on VLSI Circuits
, 2019
Ping-Wei Chen, Chi-Yang Tseng, Fumin Shi, Bo Bi, and Yu-Hwa Lo
"Detecting Protein−Ligand Interaction from Integrated Transient Induced Molecular Electronic Signal (i-TIMES)"
Analytical Chemistry
, v.92
, 2020
, p.3852
https://dx.doi.org/10.1021/acs.analchem.9b05310
Ping-Wei Chen, Chi-Yang Tseng, Fumin Shi, Bo Bi, Yu-Hwa Lo
"Measuring electric charge and Molecular coverage on electrode Surface from transient induced Molecular electronic Signal (TIMES)"
Scientific Reports
, v.9
, 2019
, p.1
https://doi.org/10.1038/s41598-019-52588-6
Tiantian Zhang, Tao Wei, Yuanyuan Han, Heng Ma, Mohammadreza Samieegohar, Ping-Wei Chen, Ian Lian, Yu-Hwa Lo
"Protein–ligand interaction detection with a novel method of transient induced molecular electronic spectroscopy (TIMES): experimental and theoretical studies"
ACS Central Science
, v.2
, 2016
, p.834
https://doi.org/10.1021/acscentsci.6b00217
PROJECT OUTCOMES REPORT
Disclaimer
This Project Outcomes Report for the General Public is displayed verbatim as submitted by the Principal Investigator (PI) for this award. Any opinions, findings, and conclusions or recommendations expressed in this Report are those of the PI and do not necessarily reflect the views of the National Science Foundation; NSF has not approved or endorsed its content.
Protein ligand interaction is one of the most fundamental and widely studied areas in biology and chemistry because of their close relation to many diseases and disease therapies. Nearly all diseases including cancer, neural disorders, infectious diseases, cardiovascular diseases, renal diseases, metabolic diseases, immune diseases, etc. are connected to the abnormality of protein-protein or protein-ligand interactions. However, all the current methods for in-vitro protein-ligand tests use either labels (often fluorescent) or ligand immobilization, both of which can produce substantial disruptions and introduce artifacts. Through the proposed research, we have developed a new technique known as transient induced molecular electronic spectroscopy (TIMES) that is both restriction-free and label-free for unperturbed measurement of these molecular interactions. We have further the TIMES technology for practical applications with high throughput by integrating ultralow noise electronics and microfluidics to form a uTIMES system with enhanced signal-to-noise ratio and throughput. We apply this method for quantitative studies of protein-ligand and protein-aptamer interactions by measuring the dissociation constant and reaction kinetics. The uTIMES system supports unperturbed measurement of the protein-ligand interaction, and in particular the dynamics of the interaction. Within each miniaturized sensor, we successfully demonstrated detection of a myriad of protein-ligand pairs with a wide range of dissociation coefficients.
In the core of the TIMES technique is its ability to measure “mobile charge” on the surface of electrode. The ability of distinguishing mobile and immobile charges on the surface over a time scale of 5-6 orders of magnitude from milliseconds to minutes is an important tribute of this method. By extending this concept and by developing an improved physical model, we have used such capabilities to measure the “absolute amount of surface charge” on the electrode surface in contact with any solution that contains any solutes or suspended nanoparticles. This “side discovery” has major impact in biosensing as it provides the only method to date, to our best knowledge, to directly quantify the surface coverage of molecules such as capture probes for the target molecules or blocking molecules for prevention of non-specific binding. The method also reveals insight on the Coulomb repelling effect and steric hindrance, both related closely to the surface charge density and ionic strength and composition of the buffer. This unique capability of the TIMES technique contributes significantly to the design and optimization of biosensors with both direct and sandwiched assays.
Last Modified: 07/30/2020
Modified by: Yu-Hwa Lo
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