2.1 Cell source.

BMSCs were obtained through generous donation by RoosterBio, Inc. (Frederick, MD, USA) at passage 2 (P2). The cells were obtained from a healthy male donor (age 31–45). The cells were screened by the company for positive adipogenic and osteogenic differentiation staining, as well as for biomarkers via flow cytometry with the following results: <5% positive for CD14, CD34, and CD45; >99% positive for CD166, CD105, CD90, and CD73. These cells are commercially referred to by the company as human bone marrow-derived mesenchymal stem cells.

2.2 Cell culture: Expansion and freezing.

BMSCs were cultured in expansion medium containing 89% low-glucose Dulbecco’s Modified Eagle Medium, 1% penicillin-streptomycin (10,000 U/mL), and 10% fetal bovine serum (FBS) lot-screened for colony formation, population doublings, and differentiation into the adipogenic and osteogenic lineages. Cells were cultured until 70% confluent, detached using trypsin-EDTA (0.05%) and cryogenically frozen as P3 in a solution of 90% FBS and 10% dimethyl sulfoxide until further use. For experiments, cells were thawed at P3 and plated at 500 cells/cm² in the same expansion medium described above. Cells were fed twice per week and, upon reaching 70% confluency, were trypsinized as P4 cells and replated for experimentation. All reagents were purchased from ThermoFisher Scientific (Waltham, MA, USA).

3.1 Cell plating density assay.

3.1.1 Motivation. To our knowledge, an assay to estimate actual plating density used in experiments involving BMSCs has not been published prior to this work. In our time lapse imaging experiments, we used glass Petri dishes rather than the traditional tissue culture polystyrene ones to optimize image quality. While we did plasma treat the glass approximately two hours prior to seeding, we hypothesized that fewer cells would attach to the dish than expected, motivating the development of a protocol to estimate actual plating density.

3.1.2 Plating into Petri dishes using limiting dilution. Petri dishes that were 60 mm in diameter and that each contained a glass well 35 mm diameter were plasma treated for 10 minutes using a plasma chamber (Diener Electronic, Ebhausen, Germany). Dishes were then placed under a UV light in a sterile tissue culture hood for approximately two hours while cells were counted and diluted. Prior to plating, dishes were also rinsed with water to remove any dust acquired from plasma treating and to ensure the glass surface was hydrophilic.

BMSCs were expanded to 70% confluency in T-175 flasks and trypsinized as P4 cells. Following trypsin neutralization and centrifugation, the cells were counted using a standard glass hemacytometer. After counting, cells were pipetted again to ensure uniform suspension, and 10% of the cell solution was transferred to a microcentrifuge tube and diluted with expansion medium to 1 mL. Cells in the 1 mL suspension were again pipetted, and 100 μL of that 1 mL was pipetted into a new centrifuge tube and diluted to 1 mL. This process was repeated until a suspension of approximately 1,000 cells/mL was achieved (usually 3 dilutions were needed). The final suspension of cells was then plated into the glass well of a Petri dish at a theoretical density of 100 cells/cm². This entire process was then repeated for each Petri dish using a new, unique dilution, where one experiment consisted of five dishes.

3.1.3 Plating density measurements. After approximately six hours (the time at which imaging began in the main experiment), cells were fixed and stained with a 0.5% solution of crystal violet (Sigma Life Science, St. Louis, MO, USA) in 100% methanol (Sigma-Aldrich, St. Louis, MO, USA). All cells present in each dish were then counted (N = 5 dishes for each of two experiments), and the plating density was calculated by dividing the number of cells by the surface area of the glass well. Counting cells was aided by drawing a grid on the bottom of each dish in a fashion akin to a hemocytometer. In the first experiment, the plating density was 17 +/- 5 cells/cm², and in the repeat experiment the density was 29 +/- 4 cells/cm², from which we have concluded that, in our hands, a theoretical plating density of 100 cells/cm2 on glass-bottomed dishes leads to a much lower actual plating density.

3.2 Time lapse imaging.

3.2.1 Initial image acquisition. Time lapse imaging of developing colonies was conducted in two separate, identical experiments. For each experiment, BMSCs were plated into five plasma-treated glass Petri dishes in the same fashion as outlined above (see Plating into Petri Dishes using Limiting Dilution in the Cell Plating Density Assay section prior to this one). After approximately six hours, dishes were inspected to ensure cells had attached. The dishes were then assessed for how far apart individual cells were. The dish with the most isolated cells was used in time lapse imaging, and the remaining four were kept in an incubator at 5% CO₂ and cultured in parallel as positive controls of cell growth. Expansion medium was added to all dishes such that the total volume was 5 mL.

Imaging was done with the petri dish kept in a stagetop incubator (Tokai Hit, Shizuoka, Japan) set at 5% CO2 and the water bath kept filled with filtered, autoclaved water for maximum possible humidity. A temperature probe was kept submerged in the MSC expansion medium at all times as a feedback sensor so that the stagetop incubator could be kept at 37°C, and the instrument was calibrated for temperature control before each use. Imaging was done with an Olympus IX81 microscope (Olympus, Shinjuku, Tokyo, Japan) with a phase contrast 10x objective. Beginning at the top of the glass well, the dish was systematically scanned left to right, top to bottom for attached cells. Cells that were especially large and circular in morphology, reminiscent of the often-cited “Type II” morphology [8], as well as cells that had more than 2 neighbors in the field of view (FOV), were omitted from imaging; the location (microscope coordinates) of all other cells was captured using Metamorph’s Multidimensional Data Acquisition application, with the cell(s) of interest positioned at the center of the FOV. This process was carried out to capture the location of as many cells as possible over the course of one hour in an effort to begin imaging before cell division occurred, resulting in the capturing of 55 locations in one experiment and 70 locations in the second. Once the locations were recorded, a MATLAB script was used to calculate the appropriate stage coordinates such that each location had a 2x2 FOV grid (1.7 x 1.3 mm). These coordinates were saved as a text file and imported back into Metamorph. Time points were set to every fifteen minutes, and imaging began approximately 7.5 hours after initial plating.

3.2.2 Monitoring of colony development. As the BMSCs migrated and proliferated into colonies, there was a need to increase the number of fields of view (FOV) during the course of the 14-day experiments. However, because our microscope stage was limited to being able to capture 400 images per 15-minutes time point, locations being monitored needed to be omitted with each FOV expansion. This monitoring was made possible through a MATLAB script that organized images by the location they belonged to, stitched the images into a montage, and made a video (see S8 and S9 Figs). The script ran every hour in order to reduce the total number of files in the output folder of Metamorph and to ensure that any videos monitored would represent the most current state of each location.

Videos were monitored daily for colony growth. Approximately two days after initial seeding, some of the monitored cells were close to migrating out of the FOV grid, and so the number of FOVs for each location was increased from 4 (2x2 FOVs, 1.7 x 1.3 mm) to 9 (3x3 FOVs, 2.6 x 2.1 mm). Locations in which cells were proliferating slowly (or not at all) were omitted from further monitoring in this transition. This process was continued until the FOV grid needed to be expanded again to a 4x4 FOV grid (Day 4, 3.5 x 2.6 mm) and finally a 5x5 FOV grid (Day 8, 4.3 x 3.3 mm). A total of 15 monitored locations remained in each experiment after the transition to a 5x5 FOV grid, and these areas were monitored for approximately 14 days. Out of the combined 30 colonies, 28 were suitable for analysis, while the other two migrated too rapidly for single cell tracking. In two of the remaining 28 locations, the colony under development at Day 4 merged with another nearby analyzed colony by Day 7 (see colonies O1/O2 and Q1/Q2 in S1 Fig). Both experiments resulted in approximately 1.1. terabytes of raw data (phase contrast images) each.

3.3 Single-cell measurements of time lapse images.

3.3.1 Image processing and cell segmentation. Several specific and detailed steps were required in order to track cells in each colony at the single-cell level. All colonies were processed and tracked as individual datasets, and estimates for the time required of each step for a typical colony are provided. The first step consisted of masking the images in an attempt to remove all background pixels and was performed using the phase contrast reconstruction algorithm proposed by Yin and Kanade [29], which minimizes a quadratic cost function and then applies thresholding in an attempt to segment cells. All acquired phase contrast images of the 28 aforementioned locations (approximately 25,000 images per colony) were masked using high-performance clusters located at the Massachusetts Green High-Performance Computing Center (Holyoke, MA, USA).

Masked images were then run through a simple pipeline in CellProfiler version 2.0.11710 [30] that identified all objects (i.e., BMSCs and artifacts not removed in masking) in the image, converted those objects into a new image, and saved that image separately. The resulting “identified objects” (IO) image was a representation of how CellProfiler interpreted individual cells; each interpreted object was a different color, and touching cells that were not successfully segmented would appear as the same color. From there, side-by-side stacks of images–one stack of the original phase contrast images, and one stack of the identified objects images–were opened side by side in ImageJ [31]. The windows synchronization tool enabled researchers to correct the identified objects images by directly tracing the phase contrast images with the paintbrush. The following corrections were made to the identified objects images: 1) all cells present in the colony that belonged to the originating progeny had a 10-pixel white dot placed on them as a “seed” for downstream processing, 2) in the case of larger, flatter cells, the cells were outlined to connect missing pieces of the cell caused by overly-aggressive masking, and 3) cells that were touching (as shown by appearing as the same color in the identified objects images) were segmented by drawing a null-pixel (black) line 5 pixels wide between their touching borders. Cells that were touching (i.e., sharing perimeters, and therefore not easily identified as separate objects in a single static image) were often identified by researchers by flipping through several images at previous and future time points. For each colony, images corresponding to 374 15-minute time points were processed in this way and took approximately 22–70 hours per colony (depending on the size and complexity of the colony). These adjusted identified objects images were then processed in a second CellProfiler pipeline that filled in all holes created by cell outlines and eliminated any objects not seeded in the previous step (approximately 12–17 hours per colony, depending on the available memory and processing power of the computer used). These processed images were then saved, inspected to ensure they were representative of the phase contrast images (e.g., no cells were missing, and no debris was present), and then submitted to tracking in CellProfiler.

3.3.2 Tracking and measurements in CellProfiler. Images processed using the methods in the previous section were run through a simple pipeline in CellProfiler that identified primary objects, assigned those objects numbers, tracked the objects, displayed the object numbers on the images, and saved the images (approximately 22–36 hours per colony, depending on the available memory and processing power of the computer used). The resulting output file was then run through a MATLAB script (versions 2014a through 2016a; The MathWorks Inc., Natick, MA, 2000) that assigned a unique identifier to each cell (e.g., if one cell was present at day 1, it was assigned an ID of 1, and its children IDs of 2 and 3 at later time points) as well as the corresponding object number of that cell at every time point. The result was a two-dimensional matrix of object numbers, with rows corresponding to each of 374 time points and columns corresponding to each unique cell over time. Cells that did not exist at any given time point (e.g., the originating cell after it divided into two unique daughter cells) were given an object number of 0. This matrix was exported as an Excel spreadsheet for further analysis.

The resulting spreadsheet was formatted in Excel to highlight all cells with a value of 0 for ease of visualization. The spreadsheet was then inspected for tracking errors: a given column contained non-zero object numbers for all time points (rows) the corresponding cell was in existence. At the time point a column began containing zeros (signifying a supposed division), two columns previously containing zeros would begin yielding non-zero object numbers (signifying the daughter cells of the dividing cell). Any instances where this was not the case was considered an error and subject to further investigation. Further, the object number of a dividing cell at its final time point, as well as the object numbers of the corresponding daughter cells at the next time point, were noted and verified in the tracked images (which displayed the object number of each cell at each time point). Any errors found in this manner (for instance, two cells that were not properly segmented for a time point and therefore appeared in the spreadsheet as one cell disappearing without two new cells appearing) were corrected, and the image set was run through the tracking pipeline again. This process was iterative, with the total active time for correcting each colony amounting to approximately 2–3 hours (depending on the complexity of the colony and the number of initial errors), and the tracking process requiring approximately 22–36 hours for each iteration (depending on the memory and processing power available for a given computer used).

Once no apparent tracking errors were present, the images were run through a more complex tracking pipeline in CellProfiler, which included several more modules in addition to the ones in the previous pipeline. These modules measured the area occupied in each image, information about neighboring cells for each cell (where a neighbor was considered at 15 pixels away), and information about the cells’ size and shape (approximately 70–110 hours per colony, depending on the computing power of the computer used). The pipeline further saved images of the identified objects as .mat files (which, when loaded into MATLAB, yielded a 2D matrix of every pixel in the image, where the values were either 0 for a null pixel or the object number for a pixel belonging to an identified object) for further use in data visualization (see “Procedures for Data Visualization” below). The resulting output file was then run through a MATLAB script that constructed cell lineage trees (with the width of the lineage lines representative of cell spread area, developed for Whitfield et al., 2013), which were inspected for any further possible errors. Errors spotted, if any, were corrected and run through the extensive pipeline again. The occurrence of errors at this stage was rare and took less that one hour to correct (plus an additional 70–110 hours to run through CellProfiler again). The resulting output file for each colony was analyzed further using MATLAB (see “Single-Cell Time Lapse Image Analysis” in the Quantification and Statistical Analysis section below).

Overall, each colony required 4–8 weeks of full-time work (where a week here is defined as 50 hours, with 100% of time devoted to processing) in order to process 374 images per colony at the single-cell level. Together, all processed colonies are a result of the combined efforts of 25 researchers, though we note that improvements and semi-automation of the processing over this period resulted in reduced human time required for validated image processing.

3.4 Procedures for data visualization.

3.4.1 Image overlay to represent cell generation and progeny (Figs 1 and S1). During tracking, .mat files were saved for each image (time point) in a given colony. Uploading these files into MATLAB displayed a 2-D matrix representative of the image, where each entry in the matrix was a value corresponding to a pixel. The values were 0 for all null-pixels; pixels belonging to an object (cell) identified in the image through the tracking pipeline described above contained the object number in the corresponding location of the matrix. These files were required for relating the analyses of the cells (described below; see Quantification and Statistical Analysis) to the cells qualitatively seen in the original phase contrast images (see S1 Fig, Day 4 images). Using the same MATLAB script employed to construct lineage trees, the object number of each cell in the final time point analyzed was mapped to that corresponding cell’s generation and originating progeny ID.

The original phase contrast images were adjusted for brightness and contrast using GIMP (www.gimp.org). A MATLAB script then conducted the following steps to create images with overlays corresponding to cell generation and progeny presented in Figs 1 and S1) imported the adjusted phase contrast image for the final time point, 2) imported the identified objects image and corresponding .mat file described above, 3) calculated the generation and originating progeny of each cell in the image (based on the tracking output file and the code used to generate cell lineage trees), along with the cells’ corresponding object number, 4) changed the RGB color value of all pixels corresponding to a given object in the identified objects image according to either the numeric value of their generation or their progeny, and 5) overlaid a transparent version this new image on top of the phase contrast image imported.

3.4.2 Representation of whole-colony properties (Fig 2). Phase contrast images at the 672^nd time point (corresponding to the final image of Day 7) were masked using the same technique described above (see “Image Processing and Cell Segmentation” above). All cells not belonging to the colony at that time point were removed from the image using a black paintbrush in ImageJ. The images were then inverted and saved as binary images. Binary images were imported into Inkscape (www.inkscape.org), and the color of the all black pixels in a given image was changed to represent the number of originating progenies belonging to that colony (as determined by studying the corresponding time lapse video from the first time point onward).

3.4.3 Representation intracolony heterogeneity (Figs 4 and S1). For a given colony, the output file from single-cell tracking in CellProfiler (see “Tracking and Measurements in CellProfiler” above) was imported into MATLAB, and from the dataset a matrix was constructed containing the x-coordinate, y-coordinate, generation, and cell spread area of each cell at the 374^th (approximately Day 4) time point was constructed. The x- and y-coordinates of each cell were then plotted in a scatter plot, with the color of the data point representing the cell generation and the size of the data point set to be relative to the corresponding cell area. The plot was then imported into Inkscape, where rings were constructed to surround the cells, representing the number and proliferative capacity of the progeny comprising the colony. For S1 Fig, a scale bar of arbitrary length (that was consistent for each colony) was added to each glyph, and the two combined were enlarged to fit the space available. Data points corresponding to senescent cells were manually marked with a “/” (see “Classification Analyses” in the Quantification and Statistical Analysis section below).

4.1 Single-cell time lapse image analysis.

4.1.1 Description of data formatting. For a given colony, the output file generated from the tracking pipeline in CellProfiler described above was reorganized in in two general ways: by constructing an array of all raw properties measured in CellProfiler (reorganized by time and unique cell identifier), and by constructing a data table of manually-calculated cell properties based off of the raw measurements. In the former, a unique identification number was assigned to each cell using the same code used to construct cell lineage trees described above. Using this ID and the object numbers of cells at each time point, the data matrix was transformed into an array with properties as columns, time points as rows, and each matrix entry a vector containing the numeric values of a given property and time point, in order of unique cell ID. The second data set constructed was a subset of manually-calculated properties (such as the average and maximum spread area over the course of each cell’s lifetime). These properties are tabulated in S2 Table.

4.1.2 Correlation analysis. The Spearman’s rank correlation coefficient (r_s) and associated p value for each pairwise comparison for all pooled colony datasets of the manually-calculated properties described in the paragraph above were calculated using the corr function in MATLAB and are presented in S2 Table (created using Excel). For each property, appropriate filters were carefully considered so as not to skew the statistics due to unrepresentative values. For example, cells which did not have a documented lifetime–either from being a first-generation cell (and therefore an unknown birth time point), a senescent cell, or a cell that did not divide within the first four days of the experiment–were filtered out of the pooled dataset before calculating the correlation coefficient between lifetime and all other listed properties. Any filters used for each property are indicated in S2 Table. Correlation coefficients and p values are highlighted in green for any pairwise comparison whose p value passed the Bonferroni-corrected p-value threshold (1.8 x 10⁻⁴, calculated with an initial p value of 0.05, divided by 276 pairwise comparisons). All p values less than 0.05 and greater than the Bonferroni-corrected p value threshold were highlighted in blue. In the main body, statistical significance is only reported for coefficients passing the Bonferroni-corrected p-value threshold.

4.1.3 Principal component analysis (PCA). Three types of datasets were constructed and combined to form an input matrix for PCA. The first dataset consisted of all properties measured by CellProfiler for all cells (see Table 1 below), averaged over each cell’s lifetime. The second dataset also contained all properties measured by CellProfiler for all cells, but at the time point of each cell’s birth. The third dataset consisted of all manually-calculated properties present in S2 Table. All data columns created by CellProfiler that corresponded to automatic tagging of the data in each frame (e.g., object numbers, which will naturally increase with increasing number of cells in the imaged frame), properties belonging to the progeny as a whole (e.g., CellProfiler’s integrated distance property, which measures the sum of the cumulative distance migrated for a cell and all of its ancestors), or properties that were replicates (e.g., the average area calculated as part of all CellProfiler properties and the average cell area present in the manually-calculated data matrix in S2 Table) were filtered from the PCA input matrix. The table below lists all 54 properties, as measured and named by CellProfiler, that we retained for further analysis.

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Table 1. All properties measured by CellProfiler at every 15 min time point and considered in further analysis.

https://doi.org/10.1371/journal.pone.0213452.t001

PCA was conducted using the pca function in MATLAB, and plots of principal component (PC) 1 and PC2 were constructed using scatter and gscatter in MATLAB. Each cell’s data point was color-coded by the generation it belonged to, the colony it belonged to, and the cluster ID it belonged to (as determined by k-means clustering using the kmeans function, where the number of clusters was set to the square-root of N divided by 2). This analysis was performed for each individual colony as well as for all colonies pooled. Similarly, PCA was also performed with all measured CellProfiler properties at specific time points (Days 1, 2, 3, and 4) for all cells in existence at that time point in all colonies combined (S3 Fig).

4.1.4 Colony infiltration. Time lapse videos of all developing single-cell-derived colonies were studied at various speeds and directions in time to assess the general time a given colony expanded to the point of approaching nearby colonies or non-migratory cells. During this assessment, it was observed that nearby cells not belonging to the colony were migrating and infiltrating the colony borders, prompting further exploration. In order to determine which, if any, cells in a perceived colony at Day 7 did not actually belong to the originating mother cell at Day 0, an image of a colony was opened in ImageJ for the final time point of Day 7, and the time lapse video of the colony was played backwards and forwards from Day 7 to the start of the experiment until four or more infiltrating cells were identified. Such cells were marked by transparent red dots on the Day 7 phase contrast images in S1 Fig (Colonies A, D, E, F, L, P, Q2, T, and Z).

4.2 Analysis of mitotic events.

We have developed a novel method for manually tracking the mitotic events of BMSCs in time lapse imaging. For a given colony, images were masked for the first 960 time points (corresponding to ten days of development) using the methods described above (see “Image Processing and Cell Segmentation” above). Cells not belonging to the colony at each time point were then eliminated using a black paintbrush in ImageJ. In some instances, images were further corrected by eliminating cells at the periphery of the colony if they protruded significantly away from the other cells (which would drastically lower the measured confluency in a way not representative of the overall colony area). Confluency was measured at every time point by running these images through a MATLAB script that measured the area occupied by the colony’s convex hull (calculated with the bwconvhull function). As a quality control, images displaying the union convex hull were also saved, overlayed on top of the original phase contrast images, and inspected to ensure the measurements were representative of the space occupied by the colony. The area occupied by the cells in the colony was measured by running the masked images through a simple pipeline in CellProfiler that identified primary objects and measured the area occupied by objects in the image. The resulting output file was imported into MATLAB, and the center of the colony at each time point was measured as the centroid of all objects at a given time point.

The time and location of mitotic events within the colony were evaluated using a combination of ImageJ and CellProfiler. In ImageJ, two stacks of images were opened side-by-side: a stack of the original phase contrast images and a stack of images the same size containing entirely zero-value pixels. The windows synchronization tool was then utilized, which allows for simultaneous scrolling through time points as well as for making marks added by the researcher in one stack appear in the other. Researchers then flipped through time points, and for every cell division (evidenced by a cell suddenly balling up into a small sphere, followed by two cells emerging), a white dot was placed on the dividing cell with the paintbrush tool at the time point just before division. Dots were placed on the original phase contrast images, and so appeared instead on the corresponding blank image in the same location. This process was conducted for 960 time points per colony, and blank images (including those that were marked with a cell division) were saved in order of their representative time point. These images were then run through a simple pipeline in CellProfiler that identified the pixel location of each marked division for all time points. The resulting output file was then imported into MATLAB, and the distance of each mitotic event from the colony center (calculated as described above) was tabulated and plotted.

4.3 Classification analyses.

Classification processes of individual cells and colonies are described below and were used in statistical analyses described either above in “Single Cell Time Lapse Image Analysis” or below in “Whole-Colony Analysis.”

4.3.1 Senescence. For each colony, an image at 374^th time point (the final time point analyzed for single-cell time lapse imaging), which displayed the object number of each cell, was used as a reference point in determining which cells divided at future time points (referred to as the “reference image” from this point forward). Time lapsed videos as well as individual images at time points beyond the reference image were then studied extensively; each cell present in the reference image was tabulated by its object number and manually tracked in the videos and/or images. Cells that divided within the next three days after the reference image were marked as proliferative, and cells that did not divide were marked as senescent.

4.3.2 Degree of isolation. Time lapse videos of each colony were studied and scored for how isolated they were from neighboring cells as they developed. A scoring system categorized colonies with a score of 1 through 5 for the following observations: 1) the colony developed with other cells present in the 2x2 fields of view (1.7 x 1.3 mm) from the start of the experiment (neighboring cells were close enough to appear in the combined field of view but migrated out of view and therefore could not be tracked); 2) neighboring cells crawled into the combined fields of view (FOVs) within the first two days of the experiment; 3) neighboring cells were revealed when the number of FOVs was expanded from a 2x2 to a 3x3 grid (2.6 x 2.1 mm) at Day 2; 4) neighboring cells migrated into the combined FOVs after they were first expanded, approximately 2–4 days after the start of imaging; 5) neighboring cells were not revealed until the FOVs were again expanded from a 3x3 to 4x4 grid (3.5 x 2.6 mm) at Day 6.

4.3.3 Asynchronicity of cell lifetime preceding cell division. The mean and standard deviation of lifetimes for all cells belonging to all colonies existing at any time point during the single-cell analysis (i.e., within the first four days) were calculated in MATLAB. The difference in lifetimes between each cell and its twin was then calculated, and cells differing in lifetime by more than the overall standard deviation (0.27 days) were tabulated as “asynchronous” for further analysis.

4.3.4 Fast vs. slow proliferators. Lineage trees of each progeny contributing to colony formation were studied to tabulate how many cells were present at the final time point analyzed at the single-cell level. Progenies were categorized as “slow dividers” if they contained less than eight cells at the final time point (corresponding to three population doublings), “fast dividers” if they contained more than 16 cells at the final time point (corresponding to four population doublings), and “moderate dividers” if they contained 8–16 cells at the final time point. Each colony was then tabulated in terms of the number of fast, moderate, and slow dividers they comprised of (S1 Table), and each cell was classified by the type of progeny it belonged to. Similarly, all cells belonging to a colony that contained a slow-dividing progeny were tabulated.

4.3.5 t-tests on binary properties. All single-cell properties having two possibilities for a given category were compared in a t-test for all manually-calculated properties displayed in S2 Table. These comparisons of “binary” classifications are listed as follows: senescent vs proliferative cells; cells belonging to a fast-dividing progeny vs cells belonging to a slow-dividing progeny; cells classified as asynchronous with their twin vs cells that were not; cells that belonged to a colony with a slow-dividing progeny vs not; and cells that had one or two senescent daughters vs. not. For each property tested in these binary classifications, a filter was applied where applicable so as not to skew results with nonrepresentative or nonsensical data. For example, when comparing the lifetime of cells for one binary category versus the other (e.g., the lifetime of cells classified as asynchronous vs cells classified as not asynchronous), all cells not having a documented lifetime–either by not dividing over the course of the experiment or by being a 1^st-generation cell whose birth time point was unknown–were omitted from the student’s t-test. The filters applied for each property tested are listed in S2 Table. The threshold for significance was a Bonferroni-corrected p-value of 0.05 divided by the number of comparisons being made for a given filter. For example, in looking at properties of cells in terms of their parents, three properties–maximum cell spread area of the parent, cell spread area of the parent before division, and lifetime of the parent–were analyzed by excluding all 1^st- and 2^nd-generation cells (whose parents have unknown properties due to the nature of the experiment). The p-value threshold for significance for these three properties under this filter was therefore 0.05/3 = 0.167.

4.4 Whole-colony analysis.

4.4.1 Measurements. Image processing was performed on all colonies at the 672^nd time point (corresponding to seven full days of colony development) as described above (see “Representation of Whole-Colony Properties” in Method Details). For each colony, the area occupied by the colony’s convex hull was calculated in MATLAB using the bwconvexhull function, and the approximate diameter reported was calculated from this measured area. In the few cases where the colony observed at Day 7 was much larger than the fields of view, the fraction of the colony imaged was approximated by visual inspection and factored into the calculations accordingly. Similarly, the confluency of the colony was calculated as the total area occupied by the cells divided by the area of the convex hull (described in more detail in “Analysis of Mitotic Events” above). The number of neighboring colonies at Day 7 was tabulated by careful observation of the original phase contrast images at the 672^nd time point by multiple observers. All other colony-wide properties, such as the number of senescent cells at Day 4, were tabulated from the results of the classification analyses described in the previous section.

4.4.2 Statistical analysis. The Spearman’s rank correlation coefficient (r_s) and associated p-value for all combinations of pairwise comparisons for the 14 whole-colony properties described above (listed in S1 Table) was calculated using the corr function in MATLAB. The results of that analysis are reported in S1 Table, which was created using Microsoft Excel. The critical threshold for r_s was +/- 0.619 [24] using the Bonferroni-corrected p value of 0.005 (calculated with an initial p value of 0.05, divided by 105 pairwise comparisons. In the main body, statistical significance is only reported for coefficients passing the Bonferroni-corrected p-value threshold. A student’s t-test was also performed to compare single-cell-derived colonies to multi-cell-derived ones for all listed properties using the ttest2 function in MATLAB and assuming unequal variance among the experimental groups.

4.5 Generation trend calculations.

Upon studying plots of area-vs-time for individual cells in a given progeny (see Figs 5D and 7C for examples), it was observed that cells appeared to have a lower spread area with each successive generation. This prompted us to quantify this observation via the Spearman’s rank correlation coefficient for area vs. generation in each progeny. To account for cells with unusually long lifetimes or for cells that were senescent, the area of each cell was defined as the average area over the first 0.83 days (the average lifetime of all cells in all colonies at all time points). This prevented large, low-generation cells from biasing the calculated correlation coefficient to higher statistical significance. The correlation coefficient between cell generation and this modified average area was calculated for each progeny using the corr function in MATLAB.