Literature DB >> 17180207

A microfluidic system in combination with optical tweezers for analyzing rapid and reversible cytological alterations in single cells upon environmental changes.

Emma Eriksson1, Jonas Enger, Bodil Nordlander, Nika Erjavec, Kerstin Ramser, Mattias Goksör, Stefan Hohmann, Thomas Nyström, Dag Hanstorp.   

Abstract

We report on the development of an experimental platform where epi-fluorescence microscopy and optical tweezers are combined with a microfluidic system to enable the analysis of rapid cytological responses in single cells. The microfluidic system allows two different media to be merged in a Y-shaped channel. Microscale channel dimensions ensure purely laminar flow and, as a result, an environmental gradient can be created between the two media. Optical tweezers are used to move a single trapped cell repeatedly between the different environments. The cell is monitored continuously by fluorescence microscopy during the experiment. In a first experiment on yeast (Saccharomyces cerevisiae) we observed changes in cell volume as the cell was moved between environments with different osmolarity. This demonstrated that the platform allowed analysis of cytological alterations on a time scale shorter than 0.2 s. In a second experiment we observed the spatial migration of the Yap1p transcription factor fused to GFP as a cell was moved from an environment of low to high oxidative capacity. The system is universal allowing the response to numerous environmental changes to be studied on the sub second time scale in a variety of model cells. We intend to use the platform to study how the age of cells, their progression through the cell cycle, or their genetic landscape, alter their capacity (kinetics and amplitude) to respond to environmental changes.

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Year:  2006        PMID: 17180207     DOI: 10.1039/b613650h

Source DB:  PubMed          Journal:  Lab Chip        ISSN: 1473-0189            Impact factor:   6.799


  19 in total

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2.  Membrane contact sites: physical attachment between chloroplasts and endoplasmic reticulum revealed by optical manipulation.

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3.  Exploitation of physical and chemical constraints for three-dimensional microtissue construction in microfluidics.

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Journal:  Biomicrofluidics       Date:  2011-06-29       Impact factor: 2.800

4.  Real-time detection of changes in the electrophoretic mobility of a single cell induced by hyperosmotic stress.

Authors:  Pau Mestres; Dmitri Petrov
Journal:  Eur Biophys J       Date:  2011-06-28       Impact factor: 1.733

5.  Pressure-driven laminar flow switching for rapid exchange of solution environment around surface adhered biological particles.

Authors:  Peter B Allen; Graham Milne; Byron R Doepker; Daniel T Chiu
Journal:  Lab Chip       Date:  2010-01-04       Impact factor: 6.799

6.  Tightly regulated and heritable division control in single bacterial cells.

Authors:  Dan Siegal-Gaskins; Sean Crosson
Journal:  Biophys J       Date:  2008-05-09       Impact factor: 4.033

Review 7.  Beyond the bulk: disclosing the life of single microbial cells.

Authors:  Katrin Rosenthal; Verena Oehling; Christian Dusny; Andreas Schmid
Journal:  FEMS Microbiol Rev       Date:  2017-11-01       Impact factor: 16.408

8.  Using single cell cultivation system for on-chip monitoring of the interdivision timer in Chlamydomonas reinhardtii cell cycle.

Authors:  Kazunori Matsumura; Toshiki Yagi; Akihiro Hattori; Mikhail Soloviev; Kenji Yasuda
Journal:  J Nanobiotechnology       Date:  2010-09-25       Impact factor: 10.435

9.  The Dynamical Systems Properties of the HOG Signaling Cascade.

Authors:  Agnès Miermont; Jannis Uhlendorf; Megan McClean; Pascal Hersen
Journal:  J Signal Transduct       Date:  2011-02-07

10.  Integrated microfluidic device for single-cell trapping and spectroscopy.

Authors:  C Liberale; G Cojoc; F Bragheri; P Minzioni; G Perozziello; R La Rocca; L Ferrara; V Rajamanickam; E Di Fabrizio; I Cristiani
Journal:  Sci Rep       Date:  2013-02-13       Impact factor: 4.379

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