# Kinetic mechanisms of amino acid transporters

> **NIH NIH R01** · UNIVERSITY OF PENNSYLVANIA · 2020 · $405,000

## Abstract

Project Summary
 Our long-term goal is to understand the mechanism of a class of protein molecules in the membranes
of cells, which transport substances in or out of cells, such as the key nutrients amino acids and glucose. The
knowledge regarding the mechanisms of these proteins in turn enable us to pursue the pathogenic
mechanisms of certain disease processes and to develop therapies. Generally, what underlies the transporting
process is a series of conformational changes of the transporter protein. The goal of this proposal is to apply
our newly developed high-resolution fluorescence-polarization-microscope-based method to determine the
energetics and dynamics of the conformational changes of a biomedically important transporter protein found
in some pathogenic bacteria.
 Structural biology has yielded abundant protein structures, revealing the structural basis of protein
functions. However, a full understanding of a protein molecule must include both its spatial and temporal
characteristics. We thus need to go beyond studying the behaviors of a protein on a near-atomic scale in a
static manner, and study it in a dynamic manner instead. However, the required experimental information
about protein dynamics is often lacking, due to the absence of relatively general methods for reliably tracking
rapid angstrom-scale conformational changes of a protein. Generally, such small changes can be reliably and
quantitatively resolved only with such structural techniques as crystallography or Cryo-EM, which,
unfortunately, lack time resolution. Conventional light microscopy, on the other hand, may be time-resolved but
its spatial resolution had remained too low to resolve angstrom-scale protein conformational changes.
 Recently, we have successfully resolved protein conformational changes on millisecond-and-angstrom
scales by examining anisotropy of a single fluorescent label attached to a chosen segment in an examined
protein, which is known to adopt a unique orientation in each crystal structural state of the protein. With a state-
of-the-art polarization microscope and analytic analyses, we have achieved an effective angle resolution of 5-
10°. Over this range, a rotational motion of a protein molecule of an average size would cause a 1.7 - 3.5 Å
change in the chord distance. Applying this method to the transporter protein, we will determine the energetics
and kinetics of conformational changes that underlie its transporting function. Integrating the resulting dynamic
information with structural information will ultimately yield an integrated, full four-dimensional mechanistic
model that accounts for the behaviors of the transporter protein, at the precision and accuracy of the
underlying measurements. Success of our proposed study will transform the way we investigate the dynamic
mechanisms of membrane proteins including transporters, and accelerate the transition from the current,
mostly static approach of structural biology to dynamic structural biol...

## Key facts

- **NIH application ID:** 10027946
- **Project number:** 1R01DK125521-01
- **Recipient organization:** UNIVERSITY OF PENNSYLVANIA
- **Principal Investigator:** ZHE LU
- **Activity code:** R01 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2020
- **Award amount:** $405,000
- **Award type:** 1
- **Project period:** 2020-07-01 → 2024-06-30

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10027946

## Citation

> US National Institutes of Health, RePORTER application 10027946, Kinetic mechanisms of amino acid transporters (1R01DK125521-01). Retrieved via AI Analytics 2026-05-24 from https://api.ai-analytics.org/grant/nih/10027946. Licensed CC0.

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