Three-dimensional tracking of the ciliate Tetrahymena reveals the mechanism of ciliary stroke-driven helical swimming

AbstractHelical swimming in free-space is a common behavior among microorganisms, such as ciliates that are covered with thousands hair-like motile cilia, and is thought to be essential for cells to orient directly to an external stimulus. However, a direct quantification of their three-dimensional (3D) helical trajectories has not been reported, in part due to difficulty in tracking 3D swimming behavior of ciliates, especially Tetrahymena with a small, transparent cell body. Here, we conducted 3D tracking of fluorescent microbeads within a cell to directly visualize the helical swimming exhibited by Tetrahymena. Our technique showed that Tetrahymena swims along a right-handed helical path with right-handed rolling of its cell body. Using the Tetrahymena cell permeabilized with detergent treatment, we also observed that influx of Ca2+ into cilia changed the 3D-trajectory patterns of Tetrahymena swimming, indicating that the beating pattern of cilia is the determining factor in its swimming behavior.

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Modelling the motion of particles around choanoflagellates

Journal of Fluid Mechanics ◽

10.1017/s0022112002002914 ◽

2003 ◽

Vol 475 ◽

pp. 333-355 ◽

Cited By ~ 15

Author(s):

B. A. A. ORME ◽

J. R. BLAKE ◽

S. R. OTTO

Keyword(s):

Cell Body ◽

Stokes Flow ◽

Three Dimensional ◽

Plane Boundary ◽

Good Qualitative Agreement ◽

Beat Pattern ◽

A Cell ◽

Passive Tracers ◽

Main Components ◽

Particle Paths

The three-dimensional particle paths due to a helical beat pattern of the flagellum of a sessile choanoflagellate, Salpingoeca Amphoridium (SA), are modelled and compared to the experimental observations of Pettitt (2001). The organism’s main components are a flagellum and a cell body which are situated above a substrate such that the interaction between these entities is crucial in determining the fluid flow around the choanoflagellate. This flow of fluid can be characterized as Stokes flow and a flow field analogous to one created by the flagellum is generated by a distribution of stokeslets and dipoles along a helical curve.The model describing the flow considers interactions between a slender flagellum, an infinite flat plane (modelling the substrate) and a sphere (modelling the cell body). The use of image systems appropriate to Green’s functions for a sphere and plane boundary are described following the method of Higdon (1979a). The computations predict particle paths representing passive tracers from experiments and their motion illustrates overall flow patterns. Figures are presented comparing recorded experimental data with numerically generated results for a number of particle paths. The principal results show good qualitative agreement with the main characteristics of flows observed in the experimental study of Pettitt (2001).

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Functional Analysis of Induced Human Ballooned Hepatocytes in a Cell Sheet-Based Three Dimensional Model

Tissue Engineering and Regenerative Medicine ◽

10.1007/s13770-020-00297-x ◽

2021 ◽

Author(s):

Botao Gao ◽

Katsuhisa Sakaguchi ◽

Tetsuya Ogawa ◽

Yuki Kagawa ◽

Hirotsugu Kubo ◽

...

Keyword(s):

Functional Analysis ◽

Cell Sheet ◽

Three Dimensional ◽

Dimensional Model ◽

Three Dimensional Model ◽

A Cell

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A Three-Dimensional Viscous Transonic Inverse Design Method

Volume 1: Aircraft Engine; Marine; Turbomachinery; Microturbines and Small Turbomachinery ◽

10.1115/2000-gt-0525 ◽

2000 ◽

Cited By ~ 4

Author(s):

W. T. Tiow ◽

M. Zangeneh

Keyword(s):

Design Method ◽

Flow Analysis ◽

Three Dimensional ◽

Viscous Effects ◽

Flow Equations ◽

Flow Solution ◽

Turbomachinery Blades ◽

A Cell ◽

Inverse Design Method ◽

Euler Solver

The development and application of a three-dimensional inverse methodology is presented for the design of turbomachinery blades. The method is based on the mass-averaged swirl, rV~θ distribution and computes the necessary blade changes directly from the discrepancies between the target and initial distributions. The flow solution and blade modification converge simultaneously giving the final blade geometry and the corresponding steady state flow solution. The flow analysis is performed using a cell-vertex finite volume time-marching algorithm employing the multistage Runge-Kutta integrator in conjunction with accelerating techniques (local time stepping and grid sequencing). To account for viscous effects, dissipative forces are included in the Euler solver using the log-law and mixing length models. The design method can be used with any existing solver solving the same flow equations without any modifications to the blade surface wall boundary condition. Validation of the method has been carried out using a transonic annular turbine nozzle and NASA rotor 67. Finally, the method is demonstrated on the re-design of the blades.

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Parallel, linear, and subnanometric 3D tracking of microparticles with Stereo Darkfield Interferometry

Science Advances ◽

10.1126/sciadv.abe3902 ◽

2021 ◽

Vol 7 (6) ◽

pp. eabe3902

Author(s):

Martin Rieu ◽

Thibault Vieille ◽

Gaël Radou ◽

Raphaël Jeanneret ◽

Nadia Ruiz-Gutierrez ◽

...

Keyword(s):

High Precision ◽

High Throughput ◽

Single Molecule ◽

Particle Tracking ◽

Focal Plane ◽

Tracking System ◽

Three Dimensional ◽

3D Tracking ◽

Single Molecule Force Spectroscopy ◽

A New Technique

While crucial for force spectroscopists and microbiologists, three-dimensional (3D) particle tracking suffers from either poor precision, complex calibration, or the need of expensive hardware, preventing its massive adoption. We introduce a new technique, based on a simple piece of cardboard inserted in the objective focal plane, that enables simple 3D tracking of dilute microparticles while offering subnanometer frame-to-frame precision in all directions. Its linearity alleviates calibration procedures, while the interferometric pattern enhances precision. We illustrate its utility in single-molecule force spectroscopy and single-algae motility analysis. As with any technique based on back focal plane engineering, it may be directly embedded in a commercial objective, providing a means to convert any preexisting optical setup in a 3D tracking system. Thanks to its precision, its simplicity, and its versatility, we envision that the technique has the potential to enhance the spreading of high-precision and high-throughput 3D tracking.

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The Development of an Automatic Three-Dimensional Mesh Generator via Modified Ray Casting

ASME 1992 International Computers in Engineering Conference: Volume 1 — Artificial Intelligence; Expert Systems; CAD/CAM/CAE; Computers in Fluid Mechanics/Thermal Systems ◽

10.1115/cie1992-0023 ◽

1992 ◽

Author(s):

Cengiz Yeker ◽

Ibrahim Zeid

Keyword(s):

Finite Elements ◽

Cell Structure ◽

Three Dimensional ◽

Ray Casting ◽

Solid Object ◽

Casting Technique ◽

Element Size ◽

A Cell ◽

Conforming Meshes ◽

Representation Scheme

Abstract A fully automatic three-dimensional mesh generation method is developed by modifying the well-known ray casting technique. The method is capable of meshing objects modeled using the CSG representation scheme. The input to the method consists of solid geometry information, and mesh attributes such as element size. The method starts by casting rays in 3D space to classify the empty and full parts of the solid. This information is then used to create a cell structure that closely models the solid object. The next step is to further process the cell structure to make it more succinct, so that the cells close to the boundary of the solid object can model the topology with enough fidelity. Moreover, neighborhood relations between cells in the structure are developed and implemented. These relations help produce better conforming meshes. Each cell in the cell structure is identified with respect to a set of pre-defined types of cells. After the identification process, a normalization process is developed and applied to the cell structure in order to ensure that the finite elements generated from each cell conform to each other and to other elements produced from neighboring cells. The last step is to mesh each cell in the structure with valid finite elements.

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The Crystal Structure of KIO3.HIO3

Canadian Journal of Chemistry ◽

10.1139/v71-072 ◽

1971 ◽

Vol 49 (3) ◽

pp. 468-476 ◽

Cited By ~ 12

Author(s):

Lilian Y. Y. Chan ◽

F. W. B. Einstein

Keyword(s):

Crystal Structure ◽

Three Dimensional ◽

Monoclinic Space Group ◽

X Ray ◽

R Factor ◽

Octahedral Environment ◽

Distorted Octahedral ◽

Potassium Hydrogen ◽

A Cell ◽

Least Squares Techniques

The crystal structure of potassium hydrogen di-iodate (bi-iodate) KIO3.HIO3 was determined from three dimensional X-ray data collected by counter methods. The structure was refined by full-matrix least-squares techniques to a conventional R factor of 5.0 % for the 1392 observed reflexions. The salt crystallizes in the monoclinic space group P21/c with eight formula units in a cell of dimension a = 7.028(1) Å, b = 8.203(1) Å, c = 21.841(3) Å, β = 98.03(1)°.The iodate units are all basically pyramidal; weak interionic I—O contacts complete a very distorted octahedral environment around three iodine atoms. There is a capped octahedral (7-coordinate) environment around the remaining iodine atom. The I—O bonds are in the range 1.75–1.82 Å and the I—OH bonds are 1.91 and 1.95 Å, variations in length can be correlated with differences in the degree of involvement in (a) hydrogen bonding and (b) interaction with adjacent iodine atoms.

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Three-Dimensional Microfabrication System for Biodegradable Microdevices With High-Resolution and Bio-Applicability

Advances in Bioengineering ◽

10.1115/imece2005-82154 ◽

2005 ◽

Cited By ~ 1

Author(s):

Akira Yamada ◽

Fuminori Niikura ◽

Koji Ikuta

Keyword(s):

Tensile Strength ◽

Biodegradable Polymers ◽

Conventional Method ◽

Three Dimensional ◽

Single Layer ◽

Batch Process ◽

Potential Applications ◽

A Cell ◽

The One ◽

Almost All

Biodegradable polymers are employed in medicine and its further application is expected with eagerness. But the lack of an appropriate processing method retards the progress. To overcome this problem, we have developped a novel three-dimensional microfabrication system. The system design allows us the processing of the free three-dimensional micro-level forms by stacking up melted polymers from the nozzle. Different from the conventional method, we adopted a batch process to supply materials in order to eliminate the prior process that required toxic solvents. In addition, it is possible to handle almost all biodegradable thermoplastic resins by adopting this system. A single layer from the piled-up layers of extruded lines was observed to evaluate the resolution. The lateral and depth resolutions attained are 40 μm and 45 μm, respectively. Biodegradable polymers enable three-dimensional microstructures such as micro-pipes, micro-bends, and micro-coil springs to be manufactured in less than 15 min. The biocompatibility of the newly fabricated structure was evaluated using a cell line (PC12). For this purpose, a small vessel, with a transparent base, was fabricated using PLA and cells were cultivated in it. The results were then compared with the results obtained using the standard method. The mechanical strength of our microstructures was evaluated using a tensile strength test. The tensile strength of the microstructure was lower than the one obtained from the conventional method, but has enough strength for fabrication of medical devices. Our system renders it possible to produce toxic-free, as well as transparent and leakage-free devices. Our system is expected to have potential applications in optimum design and fabrication of implantable devices, especially in tissue engineering.

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Podophyllotoxin and Quercetin in Silico Derivatives Docking Analysis with Cyclooxygenase-2 and Aminopeptidase-N

10.1101/2021.02.26.433103 ◽

2021 ◽

Author(s):

A.E. Manukyan ◽

A.A. Hovhannisyan

Keyword(s):

In Silico ◽

Biological Activities ◽

Three Dimensional ◽

Aminopeptidase N ◽

Docking Analysis ◽

Quercetin Derivatives ◽

Pubchem Database ◽

A Cell ◽

Cox 2 ◽

High Level

ABSTRACTThe cyclooxygenase (COX) enzymes are tumor markers, the inhibition of which can be used in the prevention and therapy of carcinogenesis. It was found that COX-2 IS considered as targets for tumor inhibition. Aminopeptidase N (APN) is a type II membrane-bound metalloprotease associated with cancer, being identified as a cell marker on the surface of malignant myeloid cells and reached a high level of expression in progressive tumors. In anticancer therapy, plant compounds are considered that can inhibit their activity. Modeling of the COX-2 and APN enzymes was carried out on the basis of molecular models of three-dimensional structures from the PDB database [PDB ID: 5f19, 4fyq] RCSB. For docking analysis, 3D ligand models were created using MarvinSketch based on the PubChem database [CID: 5280343, 5281654]. In silico experiments, for the first time, revealed the possible interaction and inhibition of COX-2 and APN by quercetin and quercetin derivatives. Aspirin and Marimastat were taken to compare the results. Possible biological activities and possible side effects of the ligands have been identified.

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Intra- and Interspecies Variability of Single-Cell Innate Fluorescence Signature of Microbial Cell

Applied and Environmental Microbiology ◽

10.1128/aem.00608-19 ◽

2019 ◽

Vol 85 (18) ◽

Author(s):

Yutaka Yawata ◽

Tatsunori Kiyokawa ◽

Yuhki Kawamura ◽

Tomohiro Hirayama ◽

Kyosuke Takabe ◽

...

Keyword(s):

Single Cell ◽

Dimensional Space ◽

Three Dimensional ◽

Population Level ◽

Microbial Cell ◽

Physiological Status ◽

Growth Phases ◽

Content Type ◽

A Cell ◽

Three Dimensional Space

ABSTRACT Here we analyzed the innate fluorescence signature of the single microbial cell, within both clonal and mixed populations of microorganisms. We found that even very similarly shaped cells differ noticeably in their autofluorescence features and that the innate fluorescence signatures change dynamically with growth phases. We demonstrated that machine learning models can be trained with a data set of single-cell innate fluorescence signatures to annotate cells according to their phenotypes and physiological status, for example, distinguishing a wild-type Aspergillus nidulans cell from its nitrogen metabolism mutant counterpart and log-phase cells from stationary-phase cells of Pseudomonas putida. We developed a minimally invasive method (confocal reflection microscopy-assisted single-cell innate fluorescence [CRIF] analysis) to optically extract and catalog the innate cellular fluorescence signatures of each of the individual live microbial cells in a three-dimensional space. This technique represents a step forward from traditional techniques which analyze the innate fluorescence signatures at the population level and necessitate a clonal culture. Since the fluorescence signature is an innate property of a cell, our technique allows the prediction of the types or physiological status of intact and tag-free single cells, within a cell population distributed in a three-dimensional space. Our study presents a blueprint for a streamlined cell analysis where one can directly assess the potential phenotype of each single cell in a heterogenous population by its autofluorescence signature under a microscope, without cell tagging. IMPORTANCE A cell’s innate fluorescence signature is an assemblage of fluorescence signals emitted by diverse biomolecules within a cell. It is known that the innate fluoresce signature reflects various cellular properties and physiological statuses; thus, they can serve as a rich source of information in cell characterization as well as cell identification. However, conventional techniques focus on the analysis of the innate fluorescence signatures at the population level but not at the single-cell level and thus necessitate a clonal culture. In the present study, we developed a technique to analyze the innate fluorescence signature of a single microbial cell. Using this novel method, we found that even very similarly shaped cells differ noticeably in their autofluorescence features, and the innate fluorescence signature changes dynamically with growth phases. We also demonstrated that the different cell types can be classified accurately within a mixed population under a microscope at the resolution of a single cell, depending solely on the innate fluorescence signature information. We suggest that single-cell autofluoresce signature analysis is a promising tool to directly assess the taxonomic or physiological heterogeneity within a microbial population, without cell tagging.

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HiCRes: a computational method to estimate and predict the resolution of HiC libraries

10.1101/2020.09.22.307967 ◽

2020 ◽

Author(s):

Claire Marchal ◽

Nivedita Singh ◽

Ximena Corso-Díaz ◽

Anand Swaroop

Keyword(s):

Expression Patterns ◽

Three Dimensional ◽

Computational Method ◽

Mathematical Concepts ◽

Regulate Gene Expression ◽

Chromatin Interactions ◽

Genome Wide ◽

A Cell ◽

Cell Type Specific ◽

Human And Mouse

AbstractThree-dimensional (3D) conformation of the chromatin is crucial to stringently regulate gene expression patterns and DNA replication in a cell-type specific manner. HiC is a key technique for measuring 3D chromatin interactions genome wide. Estimating and predicting the resolution of a library is an essential step in any HiC experimental design. Here, we present the mathematical concepts to estimate the resolution of a library and predict whether deeper sequencing would enhance the resolution. We have developed HiCRes, a docker pipeline, by applying these concepts to human and mouse HiC libraries.

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