CIL:11924, Taricha granulosa, epithelial cell of lung. In Cell Image Library ...

Comparison of actin speckle microscopy with phalloidin staining. Primary cultures of newt lung epithelial cells were microinjected with X-rhodamine actin. Time-lapse FSM was performed on a spinning disk confocal microscope system. Light from a 50-mW Krypton-Argon ion laser (Melles Griot, OmniChrome)...

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Bibliographic Details
Main Authors: Salmon, Wendy C., Adams, Michael C., Waterman-Storer, Clare M.
Format: Dataset
Language:unknown
Published: UC San Diego Library Digital Collections 2021
Subjects:
actin cytoskeleton organization
epithelial cell of lung
actin filament polymerization
actin filament depolymerization
actin cytoskeleton
Taricha granulosa
Orca
Online Access:https://dx.doi.org/10.6075/j09z93h8
https://library.ucsd.edu/dc/object/bb1166987q
Description
Summary:Comparison of actin speckle microscopy with phalloidin staining. Primary cultures of newt lung epithelial cells were microinjected with X-rhodamine actin. Time-lapse FSM was performed on a spinning disk confocal microscope system. Light from a 50-mW Krypton-Argon ion laser (Melles Griot, OmniChrome) was delivered by a single-mode fiber optic (Point Source) to a Yokogawa spinning disk confocal scan-head (Ultra-View; PerkinElmer) on an inverted microscope (TE300 Quantum; Nikon). Excitation wavelength was selected by a filter-wheel apparatus (Sutter Instruments Co.) containing excitation filters for 488 and 568 nm (Chroma). Emission was selected by multiple bandpass dichromatic mirror and emission filter (Chroma). Images were collected by a 100x 1.4NA Plan-Apo DIC objective lens (Nikon) and captured with an Orca 2 camera (Hamamatsu). Images were collected in the ventral focal plane at 10s intervals. Following live cell imaging, cells were fixed with paraformaldehyde, permeabilized and stained with Alexa 488 ... : Preparation: living tissue; formaldehyde fixed tissue Relation to intact cell: dispersed cells in vitro Item type: recorded image Imaging mode: spinning disk confocal microscopy; fluorescent speckle microscopy Parameter imaged: fluorescence emission Source of contrast: distribution of a specific protein Visualization methods: X-Rhodamine; Alexa Fluor 488; phalloidin Processing history: background subtraction, 3X3 low pass filter, unsharp mask Data qualification: Processed;spatialmeasurements;intensitiesquantitation ...

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