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Literature DB >> 25047761

An algorithm for automated detection, localization and measurement of local calcium signals from camera-based imaging.

Kyle L Ellefsen¹, Brett Settle¹, Ian Parker², Ian F Smith³.

Abstract

Local Ca(2+) transients such as puffs and sparks form the building blocks of cellular Ca(2+) signaling in numerous cell types. They have traditionally been studied by linescan confocal microscopy, but advances in TIRF microscopy together with improved electron-multiplied CCD (EMCCD) cameras now enable rapid (>500 frames s(-1)) imaging of subcellular Ca(2+) signals with high spatial resolution in two dimensions. This approach yields vastly more information (ca. 1 Gb min(-1)) than linescan imaging, rendering visual identification and analysis of local events imaged both laborious and subject to user bias. Here we describe a routine to rapidly automate identification and analysis of local Ca(2+) events. This features an intuitive graphical user-interfaces and runs under Matlab and the open-source Python software. The underlying algorithm features spatial and temporal noise filtering to reliably detect even small events in the presence of noisy and fluctuating baselines; localizes sites of Ca(2+) release with sub-pixel resolution; facilitates user review and editing of data; and outputs time-sequences of fluorescence ratio signals for identified event sites along with Excel-compatible tables listing amplitudes and kinetics of events.

Entities: CellLine Chemical Disease Gene Species

Keywords: Algorithm; Automation; Calcium; Fluorescence; Imaging; Total internal reflection microscopy

Mesh：

Substances：
Calcium

Year: 2014 PMID： 25047761 PMCID： PMC4162823 DOI： 10.1016/j.ceca.2014.06.003

Source DB: PubMed Journal: Cell Calcium ISSN： 0143-4160 Impact factor: 6.817

29 in total

1. Timescales of IP(3)-evoked Ca(2+) spikes emerge from Ca(2+) puffs only at the cellular level.

Authors: Kevin Thurley; Ian F Smith; Stephen C Tovey; Colin W Taylor; Ian Parker; Martin Falcke
Journal: Biophys J Date: 2011-12-07 Impact factor: 4.033

2. Automated detection of elementary calcium release events using the á trous wavelet transform.

Authors: F v Wegner; M Both; R H A Fink
Journal: Biophys J Date: 2005-12-30 Impact factor: 4.033

3. Automated region of interest analysis of dynamic Ca²+ signals in image sequences.

Authors: Michael Francis; Xun Qian; Chimène Charbel; Jonathan Ledoux; J C Parker; Mark S Taylor
Journal: Am J Physiol Cell Physiol Date: 2012-04-25 Impact factor: 4.249

4. Multidimensional detection and analysis of Ca2+ sparks in cardiac myocytes.

Authors: Mark-Anthony Bray; Nicholas A Geisse; Kevin Kit Parker
Journal: Biophys J Date: 2007-03-16 Impact factor: 4.033

5. The probability of triggering calcium puffs is linearly related to the number of inositol trisphosphate receptors in a cluster.

Authors: George D Dickinson; Divya Swaminathan; Ian Parker
Journal: Biophys J Date: 2012-04-18 Impact factor: 4.033

Review 6. Cytosolic Ca2+ buffers.

Authors: Beat Schwaller
Journal: Cold Spring Harb Perspect Biol Date: 2010-10-13 Impact factor: 10.005

7. Ca(2+) puffs originate from preestablished stable clusters of inositol trisphosphate receptors.

Authors: Ian F Smith; Steven M Wiltgen; Jianwei Shuai; Ian Parker
Journal: Sci Signal Date: 2009-11-24 Impact factor: 8.192

8. Localization of puff sites adjacent to the plasma membrane: functional and spatial characterization of Ca2+ signaling in SH-SY5Y cells utilizing membrane-permeant caged IP3.

Authors: Ian F Smith; Steven M Wiltgen; Ian Parker
Journal: Cell Calcium Date: 2008-07-17 Impact factor: 6.817

9. Automated detection and analysis of Ca(2+) sparks in x-y image stacks using a thresholding algorithm implemented within the open-source image analysis platform ImageJ.

Authors: Elliot M Steele; Derek S Steele
Journal: Biophys J Date: 2014-02-04 Impact factor: 4.033

10. Properties of Ca2+ sparks revealed by four-dimensional confocal imaging of cardiac muscle.

Authors: Vyacheslav M Shkryl; Lothar A Blatter; Eduardo Ríos
Journal: J Gen Physiol Date: 2012-02-13 Impact factor: 4.086

40 in total

1. Applications of FLIKA, a Python-based image processing and analysis platform, for studying local events of cellular calcium signaling.

Authors: Kyle L Ellefsen; Jeffrey T Lock; Brett Settle; Carley A Karsten; Ian Parker
Journal: Biochim Biophys Acta Mol Cell Res Date: 2018-11-27 Impact factor: 4.739

An algorithm for automated detection, localization and measurement of local calcium signals from camera-based imaging.

1. Timescales of IP(3)-evoked Ca(2+) spikes emerge from Ca(2+) puffs only at the cellular level.

2. Automated detection of elementary calcium release events using the á trous wavelet transform.

3. Automated region of interest analysis of dynamic Ca²+ signals in image sequences.

4. Multidimensional detection and analysis of Ca2+ sparks in cardiac myocytes.

5. The probability of triggering calcium puffs is linearly related to the number of inositol trisphosphate receptors in a cluster.

Review 6. Cytosolic Ca2+ buffers.

7. Ca(2+) puffs originate from preestablished stable clusters of inositol trisphosphate receptors.

8. Localization of puff sites adjacent to the plasma membrane: functional and spatial characterization of Ca2+ signaling in SH-SY5Y cells utilizing membrane-permeant caged IP3.

9. Automated detection and analysis of Ca(2+) sparks in x-y image stacks using a thresholding algorithm implemented within the open-source image analysis platform ImageJ.

10. Properties of Ca2+ sparks revealed by four-dimensional confocal imaging of cardiac muscle.

1. Applications of FLIKA, a Python-based image processing and analysis platform, for studying local events of cellular calcium signaling.

2. Imaging local Ca2+ signals in cultured mammalian cells.

3. CellSpecks: A Software for Automated Detection and Analysis of Calcium Channels in Live Cells.

4. TraceSpecks: A Software for Automated Idealization of Noisy Patch-Clamp and Imaging Data.

5. All three IP₃ receptor isoforms generate Ca²⁺ puffs that display similar characteristics.

6. Improved Methods to Detect Low Levels of HIV Using Antibody-Based Technologies.

7. Comparison of Ca²⁺ puffs evoked by extracellular agonists and photoreleased IP₃.

8. Noise analysis of cytosolic calcium image data.

Review 9. Spatial-temporal patterning of Ca²⁺ signals by the subcellular distribution of IP₃ and IP₃ receptors.

10. A comparison of fluorescent Ca²⁺ indicators for imaging local Ca²⁺ signals in cultured cells.

Review 6. Cytosolic Ca2+ buffers.

Review 9. Spatial-temporal patterning of Ca2+ signals by the subcellular distribution of IP3 and IP3 receptors.

Review 9. Spatial-temporal patterning of Ca²⁺ signals by the subcellular distribution of IP₃ and IP₃ receptors.