It has emerged that small details between in vivo and in vitro studies make for big differences in understanding diabetes and other secretory dysfunctions
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The unexpected findings that exocytosis regulation "in vivo" is not the same as the process long studied "in vitro" is a reminder of the gap between laboratory glassware experiments and the cell biology of living animals ⎯ and humans, said Roberto Weigert, Ph.D., of the National Institutes of Health (NIH), National Institute of Dental and Craniofacial Research (NIDCR).
During exocytosis, a cell internally packs up secretions and ferries them to the plasma membrane (PM) that demarcates the cell from its surroundings.
There, the packages, which are named secretory vesicles, fuse with the PM and then eject their contents. The process has been studied for decades in glassware experiments involving cultured cells and tissues.
Thanks to the optical imaging technology intravital microscopy. Weigert and colleagues were able to determine for the first time how exocytosis actually occurs in the salivary glands of a living mouse.
According to previous in vitro studies in the salivary glands, multiple secretory vesicles fuse with the PM, forming strings of vesicles in a process stimulated by two classes of chemical switches, muscarinic and beta-adrenergic receptors.
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Their additional in vivo studies revealed that the fusion step requires the assembly of a scaffold around the membrane of the vesicles.
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The molecular differences between in vivo and in vitro may seem minor but may have a large impact, said Weigert, because exocytosis is fundamental to understanding the basis of secretory dysfunctions such as diabetes in which insulin is transported in secretory vesicles.
Source-Eurekalert