Please use this identifier to cite or link to this item: http://hdl.handle.net/1942/35935
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dc.contributor.authorKazwiny, Y-
dc.contributor.authorPedrosa, J-
dc.contributor.authorZhang , ZQ-
dc.contributor.authorBOESMANS, Werend-
dc.contributor.authorD'hooge, J-
dc.contributor.authorVanden Berghe , P-
dc.date.accessioned2021-11-29T15:33:21Z-
dc.date.available2021-11-29T15:33:21Z-
dc.date.issued2021-
dc.date.submitted2021-09-13T14:46:17Z-
dc.identifier.citationScientific reports (Nature Publishing Group), 11 (1) (Art N° 10937)-
dc.identifier.urihttp://hdl.handle.net/1942/35935-
dc.description.abstractCa2+ imaging is a widely used microscopy technique to simultaneously study cellular activity in multiple cells. The desired information consists of cell-specific time series of pixel intensity values, in which the fluorescence intensity represents cellular activity. For static scenes, cellular signal extraction is straightforward, however multiple analysis challenges are present in recordings of contractile tissues, like those of the enteric nervous system (ENS). This layer of critical neurons, embedded within the muscle layers of the gut wall, shows optical overlap between neighboring neurons, intensity changes due to cell activity, and constant movement. These challenges reduce the applicability of classical segmentation techniques and traditional stack alignment and regions-of-interest (ROIs) selection workflows. Therefore, a signal extraction method capable of dealing with moving cells and is insensitive to large intensity changes in consecutive frames is needed. Here we propose a b-spline active contour method to delineate and track neuronal cell bodies based on local and global energy terms. We develop both a single as well as a double-contour approach. The latter takes advantage of the appearance of GCaMP expressing cells, and tracks the nucleus' boundaries together with the cytoplasmic contour, providing a stable delineation of neighboring, overlapping cells despite movement and intensity changes. The tracked contours can also serve as landmarks to relocate additional and manually-selected ROIs. This improves the total yield of efficacious cell tracking and allows signal extraction from other cell compartments like neuronal processes. Compared to manual delineation and other segmentation methods, the proposed method can track cells during large tissue deformations and high-intensity changes such as during neuronal firing events, while preserving the shape of the extracted Ca2+ signal. The analysis package represents a significant improvement to available Ca2+ imaging analysis workflows for ENS recordings and other systems where movement challenges traditional Ca2+ signal extraction workflows.-
dc.description.sponsorshipThe authors thank Tobie Martens for manual cell delineation and ROI selection on Ca2+ recordings. such there was no direct use of animal tissues for this study. All microscopy recordings in this study were re-used recordings from previous projects performed according to the guidelines and procedures as approved by the Animal Ethics committee of KU Leuven. The authors’ work is supported by the Research Foundation Flanders (FWO) grant G.0929.15, G.OH1816N and I001918N and Hercules AKUL/11/37 and AKUL/15/37 (to P.V.B.).-
dc.language.isoen-
dc.publisherNATURE RESEARCH-
dc.rightsThe Author(s) 2021 Open Access Tis article is licensed under a Creative Commons Attribution 4.0 International License, which permits use, sharing, adaptation, distribution and reproduction in any medium or format, as long as you give appropriate credit to the original author(s) and the source, provide a link to the Creative Commons licence, and indicate if changes were made. Te images or other third party material in this article are included in the article’s Creative Commons licence, unless indicated otherwise in a credit line to the material. If material is not included in the article’s Creative Commons licence and your intended use is not permitted by statutory regulation or exceeds the permitted use, you will need to obtain permission directly from the copyright holder. To view a copy of this licence, visit http://creativecommons.org/licenses/by/4.0/.-
dc.subject.otherAlgorithms-
dc.subject.otherAnimals-
dc.subject.otherCalcium-
dc.subject.otherCell Tracking-
dc.subject.otherEnteric Nervous System-
dc.subject.otherHumans-
dc.subject.otherImage Processing, Computer-Assisted-
dc.subject.otherMicroscopy, Fluorescence-
dc.subject.otherMuscle Contraction-
dc.subject.otherNeurons-
dc.titleExtracting neuronal activity signals from microscopy recordings of contractile tissue using B-spline Explicit Active Surfaces (BEAS) cell tracking-
dc.typeJournal Contribution-
dc.identifier.issue1-
dc.identifier.volume11-
local.format.pages14-
local.bibliographicCitation.jcatA1-
local.publisher.placeHEIDELBERGER PLATZ 3, BERLIN, 14197, GERMANY-
local.type.refereedRefereed-
local.type.specifiedArticle-
local.bibliographicCitation.artnr10937-
dc.identifier.doi10.1038/s41598-021-90448-4-
dc.identifier.pmid34035411-
dc.identifier.isi000659136700025-
local.provider.typeWeb of Science-
local.uhasselt.internationalyes-
item.fullcitationKazwiny, Y; Pedrosa, J; Zhang , ZQ; BOESMANS, Werend; D'hooge, J & Vanden Berghe , P (2021) Extracting neuronal activity signals from microscopy recordings of contractile tissue using B-spline Explicit Active Surfaces (BEAS) cell tracking. In: Scientific reports (Nature Publishing Group), 11 (1) (Art N° 10937).-
item.accessRightsOpen Access-
item.contributorKazwiny, Y-
item.contributorPedrosa, J-
item.contributorZhang , ZQ-
item.contributorBOESMANS, Werend-
item.contributorD'hooge, J-
item.contributorVanden Berghe , P-
item.fulltextWith Fulltext-
item.validationecoom 2022-
crisitem.journal.issn2045-2322-
crisitem.journal.eissn2045-2322-
Appears in Collections:Research publications
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