The CellBorderTracker, a novel tool to quantitatively analyze spatiotemporal endothelial junction dynamics at the subcellular level

Jochen Seebach; Abdallah Abu Taha; Janine Lenk; Nico Lindemann; Xiaoyi Jiang; Klaus Brinkmann; Sven Bogdan; Hans-Joachim Schnittler

doi:10.1007/s00418-015-1357-8

The CellBorderTracker, a novel tool to quantitatively analyze spatiotemporal endothelial junction dynamics at the subcellular level

Histochem Cell Biol. 2015 Dec;144(6):517-32. doi: 10.1007/s00418-015-1357-8. Epub 2015 Aug 15.

Authors

Jochen Seebach¹, Abdallah Abu Taha², Janine Lenk³, Nico Lindemann², Xiaoyi Jiang⁴, Klaus Brinkmann⁵, Sven Bogdan⁵, Hans-Joachim Schnittler⁶

Affiliations

¹ Institute of Anatomy and Vascular Biology, Westfälische Wilhelms-Universität Münster, Vesaliusweg 2-4, 48149, Münster, Germany. seebach@uni-muenster.de.
² Institute of Anatomy and Vascular Biology, Westfälische Wilhelms-Universität Münster, Vesaliusweg 2-4, 48149, Münster, Germany.
³ Faculty of Medicine Carl Gustav Carus, Fetscherstrasse 74, 01307, Dresden, Germany.
⁴ Department of Computer Science, Westfälische Wilhelms-Universität Münster, Münster, Germany.
⁵ Institute for Neurobiology, Westfälische Wilhelms-Universität Münster, Münster, Germany.
⁶ Institute of Anatomy and Vascular Biology, Westfälische Wilhelms-Universität Münster, Vesaliusweg 2-4, 48149, Münster, Germany. hans.schnittler@uni-muenster.de.

PMID: 26275669
DOI: 10.1007/s00418-015-1357-8

Abstract

Endothelial junctions are dynamic structures organized by multi-protein complexes that control monolayer integrity, homeostasis, inflammation, cell migration and angiogenesis. Newly developed methods for both the genetic manipulation of endothelium and microscopy permit time-lapse recordings of fluorescent proteins over long periods of time. Quantitative data analyses require automated methods. We developed a software package, the CellBorderTracker, allowing quantitative analysis of fluorescent-tagged cell junction protein dynamics in time-lapse sequences. The CellBorderTracker consists of the CellBorderExtractor that segments cells and identifies cell boundaries and mapping tools for data extraction. The tool is illustrated by analyzing fluorescent-tagged VE-cadherin the backbone of adherence junctions in endothelium. VE-cadherin displays high dynamics that is forced by junction-associated intermittent lamellipodia (JAIL) that are actin driven and WASP/ARP2/3 complex controlled. The manual segmentation and the automatic one agree to 90 %, a value that indicates high reliability. Based on segmentations, different maps were generated allowing more detailed data extraction. This includes the quantification of protein distribution pattern, the generation of regions of interest, junction displacements, cell shape changes, migration velocities and the visualization of junction dynamics over many hours. Furthermore, we demonstrate an advanced kymograph, the J-kymograph that steadily follows irregular cell junction dynamics in time-lapse sequences for individual junctions at the subcellular level. By using the CellBorderTracker, we demonstrate that VE-cadherin dynamics is quickly arrested upon thrombin stimulation, a phenomenon that was largely due to transient inhibition of JAIL and display a very heterogeneous subcellular and divers VE-cadherin dynamics during intercellular gap formation and resealing.

Keywords: ARP2/3 complex; Endothelial junction dynamics; Fluorescence live cell imaging; Image analysis; Inflammation; VE-cadherin.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Cadherins / analysis*
Cadherins / metabolism
Cells, Cultured
Drosophila
Endothelium, Vascular / cytology*
Endothelium, Vascular / metabolism
Fluorescence
Fluorescent Antibody Technique
Humans
Intercellular Junctions / chemistry
Intercellular Junctions / metabolism*
Software*

Substances

Cadherins