Attempts at the Characterization of In-Cell Biophysical Processes Non-Invasively-Quantitative NMR Diffusometry of a Model Cellular System

Weronika Mazur; Artur T Krzyżak

doi:10.3390/cells9092124

Attempts at the Characterization of In-Cell Biophysical Processes Non-Invasively-Quantitative NMR Diffusometry of a Model Cellular System

Cells. 2020 Sep 19;9(9):2124. doi: 10.3390/cells9092124.

Authors

Weronika Mazur^{1

2}, Artur T Krzyżak²

Affiliations

¹ Faculty of Physics and Applied Computer Science, AGH University of Science and Technology, ul. Reymonta 19, 30-059 Cracow, Poland.
² Faculty of Geology, Geophysics and Environmental Protection, AGH University of Science and Technology, al. Mickiewicza 30, 30-059 Cracow, Poland.

Abstract

In the literature, diffusion studies of cell systems are usually limited to two water pools that are associated with the extracellular space and the entire interior of the cell. Therefore, the time-dependent diffusion coefficient contains information about the geometry of these two water regions and the water exchange through their boundary. This approach is due to the fact that most of these studies use pulse techniques and relatively low gradients, which prevents the achievement of high b-values. As a consequence, it is not possible to register the signal coming from proton populations with a very low bulk or apparent self-diffusion coefficient, such as cell organelles. The purpose of this work was to obtain information on the geometry and dynamics of water at a level lower than the cell size, i.e., in cellular structures, using the time-dependent diffusion coefficient method. The model of the cell system was made of baker's yeast (Saccharomyces cerevisiae) since that is commonly available and well-characterized. We measured characteristic fresh yeast properties with the application of a compact Nuclear Magnetic Resonance (NMR)-Magritek Mobile Universal Surface Explorer (MoUSE) device with a very high, constant gradient (~24 T/m), which enabled us to obtain a sufficient stimulated echo attenuation even for very short diffusion times (0.2-40 ms) and to apply very short diffusion encoding times. In this work, due to a very large diffusion weighting (b-values), splitting the signal into three components was possible, among which one was associated only with cellular structures. Time-dependent diffusion coefficient analysis allowed us to determine the self-diffusion coefficients of extracellular fluid, cytoplasm and cellular organelles, as well as compartment sizes. Cellular organelles contributing to each compartment were identified based on the random walk simulations and approximate volumes of water pools calculated using theoretical sizes or molar fractions. Information about different cell structures is contained in different compartments depending on the diffusion regime, which is inherent in studies applying extremely high gradients.

Keywords: constant gradient; in-cell diffusion; time-dependent diffusion coefficient.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Cell Compartmentation
Cell Wall / chemistry*
Cell Wall / ultrastructure
Computer Simulation
Cytoplasm / chemistry*
Cytoplasm / ultrastructure
Diffusion
Magnetic Resonance Spectroscopy / methods
Models, Chemical
Organelles / chemistry
Organelles / ultrastructure*
Saccharomyces cerevisiae / chemistry*
Saccharomyces cerevisiae / ultrastructure
Water

Substances

Water