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Functional Microendoscopy Reveals Calcium Responses of Single Cells in Tracheal Tuft Cells and Kidney Podocytes
Author(s) -
Dancker Tobias A.,
Elhawy Mohamed Ibrahem,
Rittershauß Ramona,
Tian Qinghai,
Schwarz Yvonne,
Hoffmann Markus D. A.,
Carlein Christopher,
Wyatt Amanda,
Wahl Vanessa,
Speyerer Daniel,
Kandah Alaa,
Boehm Ulrich,
Prates Roma Leticia,
Bruns Dieter,
Lipp Peter,
KrastevaChrist Gabriela,
Lauterbach Marcel A.
Publication year - 2025
Publication title -
small
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 3.785
H-Index - 236
eISSN - 1613-6829
pISSN - 1613-6810
DOI - 10.1002/smll.202411341
Subject(s) - in vivo , tuft , flexibility (engineering) , microbiology and biotechnology , biomedical engineering , biology , biophysics , anatomy , materials science , medicine , composite material , statistics , mathematics
Abstract Microendoscopy, a crucial technology for minimally invasive investigations of organs, facilitates studies within confined cavities. However, conventional microendoscopy is often limited by probe size and the constraint of using a single excitation wavelength. In response to these constraints, a multichannel microendoscope with a slender profile of only 360 µm is engineered. Functional signals both in situ and in vivo are successfully captured from individual single cells, employing a specially developed software suite for image processing, and exhibiting an effective resolution of 4.6 µm, allowing for the resolution of subcellular neuronal structures. This system enabled the first examination of calcium dynamics in vivo in murine tracheal tuft cells (formerly named brush cells) and in situ in kidney podocytes. Additionally, it recorded ratiometric redox reactions in various biological settings, including intact explanted organs and pancreatic islet cultures. The flexibility and streamlined operation of the microendoscopic technique open new avenues for conducting in vivo research, allowing for studies of tissue and organ function at cellular resolution.
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