Informace o publikaci

Quantitative Assessment of Anti-Cancer Drug Efficacy From Coregistered Mass Spectrometry and Fluorescence Microscopy Images of Multicellular Tumor Spheroids

Logo poskytovatele
Logo poskytovatele
Autoři

MICHÁLEK Jan ŠTĚPKA Karel KOZUBEK Michal NAVRÁTILOVÁ Jarmila PAVLATOVSKÁ Barbora MACHÁLKOVÁ Markéta PREISLER Jan PRUŠKA Adam

Rok publikování 2019
Druh Článek v odborném periodiku
Časopis / Zdroj Microscopy and Microanalysis
Fakulta / Pracoviště MU

Fakulta informatiky

Citace
www http://dx.doi.org/10.1017/S1431927619014983
Doi http://dx.doi.org/10.1017/S1431927619014983
Klíčová slova confocal microscopy; image registration; MALDI MS; mass spectrometry imaging; peeling
Popis Spheroids—three-dimensional aggregates of cells grown from a cancer cell line—represent a model of living tissue for chemotherapy inves- tigation. Distribution of chemotherapeutics in spheroid sections was determined using the matrix-assisted laser desorption/ionization mass spectrometry imaging (MALDI MSI). Proliferating or apoptotic cells were immunohistochemically labeled and visualized by laser scanning confocal fluorescence microscopy (LSCM). Drug efficacy was evaluated by comparing coregistered MALDI MSI and LSCM data of drug- treated spheroids with LSCM only data of untreated control spheroids. We developed a fiducial-based workflow for coregistration of low- resolution MALDI MS with high-resolution LSCM images. To allow comparison of drug and cell distribution between the drug-treated and untreated spheroids of different shapes or diameters, we introduced a common diffusion-related coordinate, the distance from the spheroid boundary. In a procedure referred to as “peeling”, we correlated average drug distribution at a certain distance with the average reduction in the affected cells between the untreated and the treated spheroids. This novel approach makes it possible to differentiate between peripheral cells that died due to therapy and the innermost cells which died naturally. Two novel algorithms—for MALDI MS image denoising and for weighting of MALDI MSI and LSCM data by the presence of cell nuclei—are also presented.
Související projekty:

Používáte starou verzi internetového prohlížeče. Doporučujeme aktualizovat Váš prohlížeč na nejnovější verzi.

Další info