Extended live imaging with Neurog3-RFP reporter reveals the dynamics of progenitor cell cycle and differentiation.

<p>(A) Scheme summarizing the genetic strategy to visualize PDX1⁺ pancreatic progenitors and <i>NEUROG3</i>⁺ endocrine progenitors for live imaging. (B) Model of pancreatic progenitor divisions with a <i>Neurog3-RFP</i> reporter. After second division of self-renewing progenitors, cell cycle length can be obtained. Using the <i>Neurog3-RFP</i> reporter, endocrine differentiation timing and synchrony can be obtained. (C) Still images from <a href="http://www.plosbiology.org/article/info:doi/10.1371/journal.pbio.1002111#pbio.1002111.s019" target="_blank">S6 Movie</a>, demonstrating an asymmetric (P/R) division producing one Neurog3-RFP⁺ daughter and two other granddaughters (white spots) from a <i>Pdx1</i>^<i>tTA/+</i>;<i>tetO-H2B-GFP;Neurog3-RFP</i> explant. After the first division, one daughter turns on RFP (before elapsed time 30:00), and later the other daughter divides, producing two granddaughters (at elapsed time 42:12). (D-G) Images of fixed explant with native GFP (D) and immunostained for SOX9/aPKC (E) and Neurog3-RFP (F, staining for MYC-tag). White spots correspond to cells in (C), and one is RFP⁺ and two granddaughters are SOX9⁺ (E,F). Inset in (E) shows high magnification image of SOX9 staining. (H) Still images from <a href="http://www.plosbiology.org/article/info:doi/10.1371/journal.pbio.1002111#pbio.1002111.s020" target="_blank">S7 Movie</a>, demonstrating a symmetric (R/R) division producing two Neurog3-RFP⁺ daughters (grey spots). After the division, both daughters turn on RFP. (I–M) Images of fixed explant with native GFP (I) and immunostained for SOX9/aPKC (J), NEUROG3 (K), and Neurog3-RFP (L, staining for MYC-tag). Both daughters are NEUROG3⁺/RFP⁺. (N) Fraction of RFP-producing cell divisions. Each category (pink, blue, and purple bars) was counted from three movies. (O) Analysis of RFP emergence from three live imaging movies. In three cases, RFP⁺ cells divided producing two RFP⁺ cells each (cyan bar), and the majority of RFP⁺ cells were either lost or moved out of frame during back-tracking (indeterminable, purple bar). (P) Fraction of asymmetric versus symmetric cell divisions from three different measurements: NEUROG3 tracking, Neurog3-RFP tracking, and in vivo clonal analysis. All three measurements exhibit equivalent rates of divisions. Numbering denotes elapsed time in h:min, and in the cell division diagrams P indicates progenitor and R, Neurog3-RFP (C, H). Scale bars, 20 μm. Histograms and error bars represent the mean and standard deviation (<i>n</i> = 3). See <a href="http://www.plosbiology.org/article/info:doi/10.1371/journal.pbio.1002111#pbio.1002111.s027" target="_blank">S6 Table</a> for further data.</p>