Exploring the Galectin Network by Light and Fluorescence Microscopy
- PMID: 35320533
- DOI: 10.1007/978-1-0716-2055-7_17
Exploring the Galectin Network by Light and Fluorescence Microscopy
Abstract
Dynamic changes of a cell's glycophenotype are increasingly interpreted as shifts in the capacity to interact with tissue (endogenous) lectins. The status of glycan branching or chain length (e.g., core 1 vs core 2 mucin-type O-glycans and polyLacNAc additions) as well as of sialylation/sulfation has been delineated to convey signals. They are "read" by galectins, for example regulating lattice formation on the membrane and cell growth. Owing to the discovery of the possibility that these effectors act in networks physiologically resulting in functional antagonism or cooperation, their detection and distribution profiling need to be expanded from an individual (single) protein to the-at best-entire family. How to work with non-cross-reactive antibodies and with the labeled tissue-derived proteins (used as probes) is exemplarily documented for chicken and human galectins including typical activity and specificity controls. This description intends to inspire the systematic (network) study of members of a lectin family and also the application of tissue proteins beyond a single lectin category in lectin histochemistry.
Keywords: Glycocluster; Glycoprotein; Glycosylation; Histochemistry; Sialylation.
© 2022. Springer Science+Business Media, LLC, part of Springer Nature.
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