Marit H. Aure scite author profile

Summary Current dogma suggests that salivary gland homeostasis is stem cell-dependent. However, the extent of stem cell contribution to salivary gland maintenance has not been determined. We have investigated acinar cell replacement during homeostasis, growth and regeneration, using an inducible CreERT2 expressed under the control of the Mist1 gene locus. Genetic labeling, followed by a chase period, showed that acinar cell replacement is not driven by the differentiation of unlabeled stem cells. Analysis using R26Brainbow2.1 reporter revealed continued proliferation and clonal expansion of terminally differentiated acinar cells in all major salivary glands. Induced injury also demonstrated the regenerative potential of pre-labeled acinar cells. Our results support a revised model for salivary gland homeostasis based predominantly on self-duplication of acinar cells, rather than on differentiation of stem cells. The proliferative capacity of differentiated acinar cells may prove critical in the implementation of cell-based strategies to restore the salivary glands.

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Limited Regeneration of Adult Salivary Glands after Severe Injury Involves Cellular Plasticity

Weng

et al. 2018

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In the adult salivary glands, the origin of replacement and regenerated acinar cells remains unclear. Although many reports describe the identification of stem cells in adult salivary glands, we have shown that differentiated acinar cells can be maintained and regenerated through self-duplication. Here, we have used genetic mouse models to further investigate acinar cell replacement and regeneration during homeostasis and after injury. Under normal conditions or after duct ligation, replacement of duct and acinar cells occurs through lineage-restricted progenitors. In contrast, after irradiation, in vivo lineage tracing shows that acinar, as well as duct, cells contribute to acinar cell regeneration, revealing that cellular plasticity is involved in salivary gland repair. Our results also indicate that even after radiation damage, several cell populations have regenerative potential for restoring salivary gland function.

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Generation of a Single-Cell RNAseq Atlas of Murine Salivary Gland Development

et al. 2020

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Summary Understanding the dynamic transcriptional landscape throughout organ development will provide a template for regenerative therapies. Here, we generated a single-cell RNA sequencing atlas of murine submandibular glands identifying transcriptional profiles that revealed cellular heterogeneity during landmark developmental events: end bud formation, branching morphogenesis, cytodifferentiation, maturation, and homeostasis. Trajectory inference analysis suggests plasticity among acinar and duct populations. We identify transcription factors correlated with acinar differentiation including Spdef, Etv1 , and Xbp1 , and loss of Ybx1 , Eno1, Sox11, and Atf4 . Furthermore, we characterize two intercalated duct populations defined by either Gfra3 and Kit , or Gstt1 . This atlas can be used to investigate specific cell functions and comparative studies predicting common mechanisms involved in development of branching organs.

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Localization of AQP5 during development of the mouse submandibular salivary gland

et al. 2011

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Aquaporin 5 (AQP5) is known to be central for salivary fluid secretion. A study of the temporal-spatial distribution of AQP5 during submandibular gland (SMG) development and in adult tissues might offer further clues to its unknown role during development. In the present work, SMGs from embryonic day (E) 14.5–18.5 and postnatal days (P) 0, 2, 5, 25, and 60 were immunostained for AQP5 and analyzed using light microscopy. Additional confocal and transmission electron microscopy were performed on P60 glands. Our results show that AQP5 expression first occurs in a scattered pattern in the late canalicular stage and becomes more prominent and organized in the terminal tubuli/pro-acinar cells towards birth. Additional apical membrane staining in the entire intralobular duct is found just prior to birth. During postnatal development, AQP5 is expressed in both the luminal and lateral membrane of pro-acinar/acinar cells. AQP5 is also detected in the basal membrane of acinar cells at P25 and P60. In the intercalated ducts at P60, the male glands show apical staining in the entire segment, while only the proximal region is positive in the female glands. These results demonstrate an evolving distribution of AQP5 during pre- and postnatal development in the mouse SMGs.

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Marit H. Aure

Salivary Gland Homeostasis Is Maintained through Acinar Cell Self-Duplication

Limited Regeneration of Adult Salivary Glands after Severe Injury Involves Cellular Plasticity

Generation of a Single-Cell RNAseq Atlas of Murine Salivary Gland Development

Localization of AQP5 during development of the mouse submandibular salivary gland

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