YAP and TAZ regulate cell volume

Perez-Gonzalez, Nicolas A.; Rochman, Nash D.; Yao, Kai; Tao, Jiaxiang; Le, Minh Tam Tran; Flanary, Shannon; Sablich, Lucia; Toler, Ben; Crentsil, Eliana; Takaesu, Felipe; Lambrus, Bram; Huang, Jessie; Fu, Vivian; Chengappa, Pragati; Jones, Tia M.; Holland, Andrew J.; An, Steven S.; Wirtz, Denis; Petrie, Ryan J.; Guan, Kun Liang; Sun, Sean X.

doi:10.1083/jcb.201902067

Cited by 41 publications

(46 citation statements)

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“…We also found that PGC1/PPAR directly regulates Yap1, a conserved transcriptional regulator of organ/cell size (Lloyd, 2013). The role of Yap1 has been extensively studied on CM proliferation for heart repair (Wang et al, 2018), but growing evidence suggests its critical role in cellular hypertrophy (Perez-Gonzalez et al, 2019;Windmueller and Morrisey, 2015). Similarly, our data showed that Yap1 is a key mediator of PGC1/PPAR for CM growth.…”

Section: Discussionmentioning

confidence: 65%

“…Calcium handling genes and ion channels including Ryr2, Atp2a2, Casq1, critical for contractility development, were continually upregulated while genes involved in cell cycle, including Cdk1, Cdk4, Ccnd1 (Mohamed et al, 2018;Yang et al, 2014), were downregulated ( Figure 1F). Conserved genes governing cellular hypertrophy, including Mtor, Yap1, Igf1r (Lloyd, 2013;Perez-Gonzalez et al, 2019), were modestly downregulated or maintained in expression as they are known to regulate cell volume ( Figure 1F). Gene ontology (GO) analysis indicated that genes related to muscle contraction and cellular metabolism are highly regulated during the process ( Figure S1A).…”

Section: Cms Exhibit High Levels Of Transcriptomic Heterogeneitymentioning

confidence: 99%

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PGC1/PPAR Drive Cardiomyocyte Maturation through Regulation of Yap1 and SF3B2

Murphy

Miyamoto

Kervadec

et al. 2020

Preprint

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Cardiomyocytes undergo significant levels of structural and functional changes after birth-fundamental processes essential for the heart to produce the volume and contractility to pump blood to the growing body. However, due to the challenges in isolating single postnatal/adult myocytes, how individual newborn cardiomyocytes acquire multiple aspects of mature phenotypes remains poorly understood. Here we implemented large-particle sorting and analyzed single myocytes from neonatal to adult hearts. Early myocytes exhibited a wide-ranging transcriptomic and size heterogeneity, maintained until adulthood with a continuous transcriptomic shift. Gene regulatory network analysis followed by mosaic gene deletion revealed that peroxisome proliferator-activated receptor coactivator-1 signaling-activated in vivo but inactive in pluripotent stem cellderived cardiomyocytes-mediates the shift. The signaling regulated key aspects of cardiomyocyte maturation simultaneously through previously unrecognized regulators, including Yap1 and SF3B2. Our study provides a single-cell roadmap of heterogeneous transitions coupled to cellular features and unveils a multifaceted regulator controlling cardiomyocyte maturation. bioRxiv | February 6, 2020 1-16

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Section: Discussionmentioning

confidence: 65%

Section: Cms Exhibit High Levels Of Transcriptomic Heterogeneitymentioning

confidence: 99%

PGC1/PPAR Drive Cardiomyocyte Maturation through Regulation of Yap1 and SF3B2

Murphy

Miyamoto

Kervadec

et al. 2020

Preprint

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“…Exclusion method (FXm), first proposed in 1983 14 and subsequently developed and refined by several groups [18][19][20] . Cells are seeded in a micro-fabricated chamber and a membrane-impermeable high molecular weight fluorescent dye (e.g.…”

Section: An Accurate and High Throughput Methods Of Cell Volume Quantimentioning

confidence: 99%

CTRL – a label-free artificial intelligence method for dynamic measurement of single-cell volume

Yao

Rochman

Sun

2020

Journal of Cell Science

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“…An accurate and high throughput method of cell volume quantification is the Fluorescence Exclusion method (FXm), first proposed in 1983 14 and subsequently developed and refined by several groups [18][19][20] . Cells are seeded in a micro-fabricated chamber and a membrane-impermeable high molecular weight fluorescent dye (e.g.…”

Section: Main Textmentioning

confidence: 99%

“…Cell suspension alters the cell shape and biochemical signaling from the extracellular matrix, and also potentially affecting cell size. None of these methods has been successfully applied to measure mammalian cell growth at the single-cell level.While sensitive and accurate methods have been developed to measure single-cell mass over time 17 , the relationship between cell size and mass is not always clear.An accurate and high throughput method of cell volume quantification is the Fluorescence Exclusion method (FXm), first proposed in 1983 14 and subsequently developed and refined by several groups [18][19][20] . Cells are seeded in a micro-fabricated chamber and a membrane-impermeable high molecular weight fluorescent dye (e.g.…”

mentioning

confidence: 99%

CTRL: a label-free method for dynamic measurement of single-cell volume

Yao

Rochman

Sun

2019

Preprint

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Measuring the physical size of the cell is valuable in understanding cell growth control. Current singlecell volume measurement methods for mammalian cells are labor-intensive, inflexible, and can cause cell damage. We introduce CTRL: Cell Topography Reconstruction Learner, a label-free technique incorporating Deep Learning and Fluorescence Exclusion for reconstructing cell topography and estimating mammalian cell volume from DIC microscopy images alone. The method achieves quantitative accuracy, requires minimal sample preparation, and applies to extensive biological and experimental conditions. Using this method, we observe a noticeable reduction in cell size fluctuations during cell cycle, which is consistent with the presence of a cell size checkpoint.(https://GitHub.com/sxslabjhu/CTRL) Main textCell size plays a critical role during cell growth, division, and proliferation 1-5 . Abnormalities in cell size regulation and growth control are thought to promote disease development 2,5-9 . Accurately measuring single-cell size remains a challenge for mammalian cells due to their irregular shape. Existing techniques require specialized hardware, fluorescent labeling 10,11 and/or cell suspension [12][13][14][15][16] . Fluorescent labeling or over-expression of a target marker can alter cell function. Cell suspension alters the cell shape and biochemical signaling from the extracellular matrix, and also potentially affecting cell size. None of these methods has been successfully applied to measure mammalian cell growth at the single-cell level.While sensitive and accurate methods have been developed to measure single-cell mass over time 17 , the relationship between cell size and mass is not always clear.An accurate and high throughput method of cell volume quantification is the Fluorescence Exclusion method (FXm), first proposed in 1983 14 and subsequently developed and refined by several groups [18][19][20] . Cells are seeded in a micro-fabricated chamber and a membrane-impermeable high molecular weight fluorescent dye (e.g. FITC-dextran) is injected into the microchamber (Fig. 1a). The cell excludes its volume in the microchamber, therefore the total fluorescence loss is proportional to the cell volume.The FXm method obtains the cell volume from a single epi-fluorescence image, and therefore is high throughput 3,18-20 . However, due to endocytosis 3,20 that is common in many cell types, the dye eventually enters the cytoplasm, and therefore FXm generally cannot accurately report cell volume in time-lapse without careful controls. Fluorescent imaging also introduces photobleaching, which alters the signal during time-lapse measurements. Moreover, microfluidic fabrication is needed to perform the experiment and the confinement of the microchamber may alter cell physiological processes over long periods. These drawbacks limit the use and applicability of FXm for studying cell growth.Convolutional Neural Networks (CNN) have been applied to microscopy images for both phenotype classification 21,22 and image segmentati...

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YAP and TAZ regulate cell volume

Cited by 41 publications

References 40 publications

PGC1/PPAR Drive Cardiomyocyte Maturation through Regulation of Yap1 and SF3B2

PGC1/PPAR Drive Cardiomyocyte Maturation through Regulation of Yap1 and SF3B2

CTRL – a label-free artificial intelligence method for dynamic measurement of single-cell volume

CTRL: a label-free method for dynamic measurement of single-cell volume

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