A OneStep Solution to Fix and Stain Cells for Correlative Live and Fixed Microscopy

Rosário, Carline Fermino do; Wadsworth, Patricia; Fritz‐Laylin, Lillian K.

doi:10.1002/cpz1.308

Cited by 4 publications

(3 citation statements)

References 11 publications

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“…S3A ) was performed live on the microscope using the OneStep fixing and staining protocol. 95 Briefly, ~2X10 4 cells (in 150 μl of M7 media) were seeded into a 96-well glass bottom plate (dot scientific, MGB096-1-2-LG-L), and imaged using DIC. During imaging, cells were treated with 150 μl of 0.2% DMSO or 10 μM LatB (for final concentrations of 0.1% DMSO and 5 μM LatB).…”

Section: Methodsmentioning

confidence: 99%

“…We verified that DMSO- and Latrunculin-treated cells continued to pump their contractile vacuoles. Then, 150 μl of solution was removed from the well and 150 μl of OneStep fixing and staining solution (100 mM sucrose, 50 mM sodium phosphate buffer, 3.6% PFA, 0.025% NP-40, DAPI, and Alexa Fluor 488 Phalloidin-488: see 95 for additional details) were added. Imaging continued, adding in fluorescence to detect actin polymer and DNA.…”

Section: Methodsmentioning

confidence: 99%

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A conserved pressure-driven mechanism for regulating cytosolic osmolarity

Garner

Beckford

Weeda

et al. 2023

Preprint

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Controlling intracellular osmolarity is essential to all cellular life. Cells that live in hypo-osmotic environments like freshwater must constantly battle water influx to avoid swelling until they burst. Many eukaryotic cells use contractile vacuoles to collect excess water from the cytosol and pump it out of the cell. Although contractile vacuoles are essential to many species, including important pathogens, the mechanisms that control their dynamics remain unclear. To identify basic principles governing contractile vacuole function, we here investigate the molecular mechanisms of two species with distinct vacuolar morphologies from different eukaryotic lineages—the discobanNaegleria gruberi, and the amoebozoan slime moldDictyostelium discoideum. Using quantitative cell biology we find that, although these species respond differently to osmotic challenges, they both use actin for osmoregulation, as well as vacuolar-type proton pumps for filling contractile vacuoles. We also use analytical modeling to show that cytoplasmic pressure is sufficient to drive water out of contractile vacuoles in these species, similar to findings from the alveolateParamecium multimicronucleatum. Because these three lineages diverged well over a billion years ago, we propose that this represents an ancient eukaryotic mechanism of osmoregulation.

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Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

A conserved pressure-driven mechanism for regulating cytosolic osmolarity

Garner

Beckford

Weeda

et al. 2023

Preprint

Self Cite

View full text Add to dashboard Cite

show abstract

“…Such systems are typically tailored for the high-resolution to super-resolution domain, custom-built, and require specialized expertise. Because of the inherent spatial resolution of this domain, such systems are difficult to calibrate and force researchers into using single-system multi-modal imaging (1, 2), with on-stage fixation and labeling protocols (1, 3, 4). On the other hand, multi-system correlative imaging (5, 6, 7, 8, 9) is dependent on finding a transformation between the respective coordinate systems.…”

Section: Introductionmentioning

confidence: 99%

Data-driven microscopy allows for automated targeted acquisition of relevant data with higher fidelity

André

Ahnlide

Norlin

et al. 2022

Preprint

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Light microscopy is a powerful single-cell technique that allows for quantitative spatial information at subcellular resolution. However, unlike flow cytometry and single-cell sequencing techniques, microscopy has issues achieving highquality population-wide sample characterization while maintaining high resolution. Here, we present a general framework, data-driven microscopy (DDM), that uses population-wide cell characterization to enable data-driven high-fidelity imaging of relevant phenotypes. DDM combines data-independent and data-dependent steps to synergistically enhance data acquired using different imaging modalities. As proof-of-concept, we apply DDM with plugins for improved high-content screening and live adaptive microscopy. DDM also allows for easy correlative imaging in other systems with a plugin that uses the spatial relationship of the sample population for automated registration. We believe DDM will be a valuable approach for reducing human bias, increasing reproducibility, and placing single-cell characteristics in the context of the sample population when interpreting microscopy data, leading to an overall increase in data fidelity.

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A OneStep Solution to Fix and Stain Cells for Correlative Live and Fixed Microscopy

2021

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Correlating the location of subcellular structures with dynamic cellular behaviors is difficult when working with organisms that lack the molecular genetic tools needed for expressing fluorescent protein fusions. Here, we describe a protocol for fixing, permeabilizing, and staining cells in a single step while imaging on a microscope. In contrast to traditional, multi‐step fixing and staining protocols that take hours, the protocol outlined here achieves satisfactory staining within minutes. This approach takes advantage of well‐characterized small molecules that stain specific subcellular structures, including nuclei, mitochondria, and actin networks. Direct visualization of the entire process allows for rapid optimization of cell fixation and staining, as well as straightforward identification of fixation artifacts. Moreover, live imaging prior to fixation reveals the dynamic history of cellular features, making it particularly useful for model systems without the capacity for expressing fluorescent protein fusions. © 2021 The Authors. Current Protocols published by Wiley Periodicals LLC. Basic Protocol: Fixing, permeabilizing, and staining mammalian cells in one step on the microscope

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A OneStep Solution to Fix and Stain Cells for Correlative Live and Fixed Microscopy

Cited by 4 publications

References 11 publications

A conserved pressure-driven mechanism for regulating cytosolic osmolarity

A conserved pressure-driven mechanism for regulating cytosolic osmolarity

Data-driven microscopy allows for automated targeted acquisition of relevant data with higher fidelity

A OneStep Solution to Fix and Stain Cells for Correlative Live and Fixed Microscopy

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