Contents

poly(A) tail length of transcripts can be measured using the PAT-Seq protocol. This protocol produces 3’-end focussed reads that include the poly(A) tail. We examine GSE83162. This is a time-series experiment in which two strains of yeast are released into synchronized cell cycling and observed through two cycles. Yeast are treated with \(\alpha\)-factor, which causes them to stop dividing in antici… pation of a chance to mate. When the \(\alpha\)-factor is washed away, they resume cycling.

1 Read files, extract experimental design from sample names

library(tidyverse)     # ggplot2, etc
library(patchwork)     # side-by-side plots
library(limma)         # differential testing
library(topconfects)   # differential testing - top confident effect sizes
library(org.Sc.sgd.db) # Yeast organism info
library(weitrix)       # Matrices with precisions weights

# Produce consistent results
set.seed(12345)

# BiocParallel supports multiple backends. 
# If the default hangs or errors, try others.
# The most reliable backed is to use serial processing
BiocParallel::register( BiocParallel::SerialParam() )
tail <- system.file("GSE83162", "tail.csv.gz", package="weitrix") %>%
    read.csv(check.names=FALSE) %>%
    column_to_rownames("Feature") %>%
    as.matrix()

tail_count <- system.file("GSE83162", "tail_count.csv.gz", package="weitrix") %>%
    read.csv(check.names=FALSE) %>%
    column_to_rownames("Feature") %>%
    as.matrix()
    
samples <- data.frame(sample=I(colnames(tail))) %>%
    extract(sample, c("strain","time"), c("(.+)-(.+)"), remove=FALSE) %>%
    mutate(
        strain=factor(strain,unique(strain)), 
        time=factor(time,unique(time)))
rownames(samples) <- colnames(tail)

samples
##                          sample    strain  time
## WT-tpre                 WT-tpre        WT  tpre
## WT-t0m                   WT-t0m        WT   t0m
## WT-t15m                 WT-t15m        WT  t15m
## WT-t30m                 WT-t30m        WT  t30m
## WT-t45m                 WT-t45m        WT  t45m
## WT-t60m                 WT-t60m        WT  t60m
## WT-t75m                 WT-t75m        WT  t75m
## WT-t90m                 WT-t90m        WT  t90m
## WT-t105m               WT-t105m        WT t105m
## WT-t120m               WT-t120m        WT t120m
## DeltaSet1-tpre   DeltaSet1-tpre DeltaSet1  tpre
## DeltaSet1-t0m     DeltaSet1-t0m DeltaSet1   t0m
## DeltaSet1-t15m   DeltaSet1-t15m DeltaSet1  t15m
## DeltaSet1-t30m   DeltaSet1-t30m DeltaSet1  t30m
## DeltaSet1-t45m   DeltaSet1-t45m DeltaSet1  t45m
## DeltaSet1-t60m   DeltaSet1-t60m DeltaSet1  t60m
## DeltaSet1-t75m   DeltaSet1-t75m DeltaSet1  t75m
## DeltaSet1-t90m   DeltaSet1-t90m DeltaSet1  t90m
## DeltaSet1-t105m DeltaSet1-t105m DeltaSet1 t105m
## DeltaSet1-t120m DeltaSet1-t120m DeltaSet1 t120m

“tpre” is the cells in an unsynchronized state, other times are minutes after release into cycling.

The two strains are a wildtype and a strain with a mutated set1 gene.

2 Create weitrix object

These tail lengths are each the average over many reads. We therefore weight each tail length by the number of reads. This is somewhat overoptimistic as there is biological noise that doesn’t go away with more reads, which we will correct for in the next step.

good <- rowMeans(tail_count) >= 10
table(good)
## good
## FALSE  TRUE 
##  1657  4875
wei <- as_weitrix(
    tail[good,,drop=FALSE], 
    weights=tail_count[good,,drop=FALSE])

rowData(wei)$gene <- AnnotationDbi::select(
    org.Sc.sgd.db, keys=rownames(wei), columns=c("GENENAME"))$GENENAME
rowData(wei)$total_reads <- rowSums(weitrix_weights(wei))
colData(wei) <- cbind(colData(wei), samples)

3 Calibration

Our first step is to calibrate our weights. Our weights are overoptimistic for large numbers of reads, as there is a biological components of noise that does not go away with more reads.

Calibration requires a model explaining non-random effects. We provide a design matrix and a weighted linear model fit is found for each row. The lack of replicates makes life difficult, for simplicity here we will assume time and strain are independent.

design <- model.matrix(~ strain + time, data=colData(wei))
fit <- weitrix_components(wei, design=design)

A gamma GLM with log link function can then be fitted to the squared residuals. 1 over the predictions from this models will serve as the new weights.

cal <- weitrix_calibrate_all(
    wei, 
    design = fit, 
    trend_formula = ~well_knotted_spline(mu,3)+well_knotted_spline(log(weight),3))
## mu range  4.402217 77.000000 knots 23.04834 30.07095 37.91549
## log(weight) range  0.0000 10.6244 knots 2.841452 4.397124 6.359334

For comparison, we’ll also look at completely unweighted residuals.

unwei <- wei
weitrix_weights(unwei) <- weitrix_weights(unwei) > 0 
# (missing data still needs weight 0)

Calibration should remove any pattern in the weighted residuals, compared to known covariates. The trend line shown in red is based on the squared weighted residuals.

First look for any pattern relative to the linear model prediction (“mu”). A trend has been removed by the calibration.

weitrix_calplot(unwei, fit, covar=mu, guides=FALSE) + labs(title="Unweighted\n") |
weitrix_calplot(wei, fit, covar=mu, guides=FALSE) + labs(title="Weighted by\nread count") |
weitrix_calplot(cal, fit, covar=mu, guides=FALSE) + labs(title="Calibrated\n")

Next look for any pattern relative to the number of reads (recall these were the original weights). Again, a trend has been removed by the calibration.

weitrix_calplot(unwei, fit, covar=log(weitrix_weights(wei)), guides=FALSE) + labs(title="Unweighted\n") |
weitrix_calplot(wei, fit, covar=log(weitrix_weights(wei)), guides=FALSE) + labs(title="Weighted by\nread count") |
weitrix_calplot(cal, fit, covar=log(weitrix_weights(wei)), guides=FALSE) + labs(title="Calibrated\n")

4 Testing

4.1 Top confident effects

We are now ready to test things.

My recommended approach is to find top confident effects, here top confident differential tail length. Core functionality is implemented in my package topconfects. Applying this to a weitrix is done using the weitrix_confects function. Rather than picking “most significant” genes, it will highlight genes with a large effect size.

weitrix_confects(cal, design, coef="strainDeltaSet1", fdr=0.05)
## $table
##    confect effect se     df    fdr_zero  row_mean typical_obs_err
## 1  -2.569  -6.027 0.6864 30.25 3.915e-06 26.23    1.485          
## 2  -2.104  -7.124 1.0472 30.25 3.538e-04 29.08    2.057          
## 3  -1.212  -5.070 0.8298 30.25 1.207e-03 14.87    1.773          
## 4  -1.064  -3.420 0.5180 30.25 4.108e-04 19.10    1.119          
## 5  -0.872  -3.470 0.5833 30.25 1.265e-03 20.29    1.267          
## 6  -0.872  -7.505 1.5042 30.25 6.497e-03 38.19    3.062          
## 7  -0.872  -3.304 0.5610 30.25 1.279e-03 18.36    1.218          
## 8  -0.872  -6.710 1.3544 30.25 6.497e-03 20.48    2.627          
## 9  -0.831  -2.867 0.4782 30.25 1.265e-03 26.88    1.055          
## 10  0.828   5.472 1.0990 30.25 6.497e-03 29.08    2.290          
##    name                gene total_reads
## 1  YDR170W-A           <NA>  4832      
## 2  YIL015W             BAR1  3898      
## 3  YAR009C             <NA>  1866      
## 4  YJR027W/YJR026W     <NA>  6577      
## 5  YML045W/YML045W-A   <NA>  4553      
## 6  YHR051W             COX6  1167      
## 7  YPL257W-B/YPL257W-A <NA>  5729      
## 8  YOR192C-B/YOR192C-A <NA>   864      
## 9  YIL053W             GPP1 25996      
## 10 YGL209W             MIG2  1937      
## ...
## 112 of 4875 non-zero contrast at FDR 0.05
## Prior df 21.2

This lists the largest confident changes in poly(A) tail length. The confect column is an inner confidence bound on the difference in tail length, adjusted for multiple testing.

Note that due to PCR amplification slippage and limited read length, the observed poly(A) tail lengths may be an underestimate. However as all samples have been prepared in the same way, observed differences should indicate the existence of true differences.

If you prefer to rank by signal to noise ratio, it is possible to use Cohen’s f as an effect size. This is similar to ranking by p-value, but Cohen’s f can be interpreted meaningfully as a signal to noise ratio.

weitrix_confects(cal, design, coef="strainDeltaSet1", effect="cohen_f", fdr=0.05)
## $table
##    confect effect strainDeltaSet1 fdr_zero  row_mean typical_obs_err
## 1  0.569   1.963  -6.027          3.915e-06 26.23    1.4851         
## 2  0.322   1.521  -7.124          3.538e-04 29.08    2.0570         
## 3  0.317   1.476  -3.420          4.108e-04 19.10    1.1193         
## 4  0.259   1.366  -5.070          1.207e-03 14.87    1.7733         
## 5  0.259   1.341  -2.867          1.265e-03 26.88    1.0552         
## 6  0.259   1.330  -3.470          1.265e-03 20.29    1.2672         
## 7  0.259   1.317  -3.304          1.279e-03 18.36    1.2180         
## 8  0.174   1.190  -2.846          5.584e-03 18.31    1.1618         
## 9  0.171   1.170  -2.804          6.426e-03 18.99    1.1637         
## 10 0.171   1.144  -2.283          6.497e-03 27.95    0.9934         
##    name                gene total_reads
## 1  YDR170W-A           <NA>  4832      
## 2  YIL015W             BAR1  3898      
## 3  YJR027W/YJR026W     <NA>  6577      
## 4  YAR009C             <NA>  1866      
## 5  YIL053W             GPP1 25996      
## 6  YML045W/YML045W-A   <NA>  4553      
## 7  YPL257W-B/YPL257W-A <NA>  5729      
## 8  YLR157C-B/YLR157C-A <NA>  5519      
## 9  YPR137C-B/YPR137C-A <NA>  7287      
## 10 YOL109W             ZEO1 34839      
## ...
## 112 of 4875 non-zero Cohen's f at FDR 0.05
## Prior df 21.2

4.2 Testing with limma

If you prefer a more traditional approach, we can feed our calibrated weitrix to limma.

fit_cal_design <- cal %>%
    weitrix_elist() %>%
    lmFit(design)

ebayes_fit <- eBayes(fit_cal_design)

topTable(ebayes_fit, "strainDeltaSet1", n=10) %>%
    dplyr::select(
        gene,diff_tail=logFC,ave_tail=AveExpr,adj.P.Val,total_reads)
##                     gene diff_tail ave_tail    adj.P.Val total_reads
## YDR170W-A           <NA> -6.027208 25.87662 3.915262e-06        4832
## YJR027W/YJR026W     <NA> -3.419778 19.40928 4.107986e-04        6577
## YIL015W             BAR1 -7.124118 30.24503 3.538329e-04        3898
## YAR009C             <NA> -5.070438 15.56624 1.207189e-03        1866
## YIL053W             GPP1 -2.867498 27.19599 1.265338e-03       25996
## YML045W/YML045W-A   <NA> -3.470070 20.55073 1.265338e-03        4553
## YPL257W-B/YPL257W-A <NA> -3.304377 18.59545 1.278512e-03        5729
## YLR157C-B/YLR157C-A <NA> -2.845888 18.46280 5.584245e-03        5519
## YPR137C-B/YPR137C-A <NA> -2.803791 19.21016 6.425669e-03        7287
## YOL109W             ZEO1 -2.282940 28.11748 6.497358e-03       34839

4.3 Testing multiple contrasts

weitrix_confects can also be used as an omnibus test of multiple contrasts. Here the default effect size will be standard deviation of observations explained by the part of the model captured by the contrasts. The standardized effect size “Cohen’s f” can also be used.

Here we will look for any step changes between time steps, ignoring the “tpre” timepoint. The exact way these contrasts are specified will not modify the ranking, so long as they specify the same subspace of coefficients.

multiple_contrasts <- limma::makeContrasts(
    timet15m-timet0m, timet30m-timet15m, timet45m-timet30m, 
    timet60m-timet45m,  timet75m-timet60m, timet90m-timet75m, 
    timet105m-timet90m, timet120m-timet105m, 
    levels=design)
## Warning in limma::makeContrasts(timet15m - timet0m, timet30m - timet15m, :
## Renaming (Intercept) to Intercept
weitrix_confects(cal, design, contrasts=multiple_contrasts, fdr=0.05)
## $table
##    confect effect timet15m - timet0m timet30m - timet15m timet45m - timet30m
## 1  3.5     5.858   -9.8373           10.8696              1.5141            
## 2  3.5     7.524   -0.3369           -0.3586              8.7815            
## 3  3.5     5.785   -0.4785            4.0872             -2.2867            
## 4  3.5     5.323   -6.8395           10.2452              0.8396            
## 5  3.4     7.410  -11.8301            7.4880              4.4171            
## 6  3.2     9.821   -8.3607            7.6550             18.4197            
## 7  2.8     6.285   -6.8300           10.1441              6.2579            
## 8  2.8     4.078    4.8376           -7.2995             -3.3326            
## 9  2.7     7.400    2.3901            6.4600             -0.1309            
## 10 2.6     3.722    2.6153            1.9706             -0.3507            
##    timet60m - timet45m timet75m - timet60m timet90m - timet75m
## 1   -0.1804             1.857               -1.2957           
## 2   -0.4211            12.594               -5.5116           
## 3    7.2778             8.972               -1.4281           
## 4    0.1190             5.537               -2.5875           
## 5    7.2070             1.792               -5.5915           
## 6  -13.1018            18.661              -13.1212           
## 7   -2.3809             4.930               -5.4150           
## 8   -0.1799             5.257                4.4367           
## 9    3.7622            11.352              -15.9122           
## 10   2.4888             3.903                0.1883           
##    timet105m - timet90m timet120m - timet105m fdr_zero  row_mean
## 1   3.97229             -0.40015              2.440e-08 29.37   
## 2   3.86528              0.20344              6.670e-06 45.91   
## 3  -0.07182             -1.28441              1.210e-07 30.67   
## 4   1.64288             -1.47056              1.231e-08 38.24   
## 5   0.76415             -0.79431              1.661e-05 29.85   
## 6  -2.41187              7.39443              2.320e-04 31.90   
## 7   2.28033             -2.57263              2.771e-05 36.33   
## 8   1.34827              0.02541              1.774e-09 14.49   
## 9  14.50129             -5.28822              2.028e-04 39.64   
## 10  1.16199             -1.69823              1.774e-09 22.41   
##    typical_obs_err name    gene   total_reads
## 1  1.833           YNL036W NCE103  5712      
## 2  3.156           YBL097W BRN1    1680      
## 3  1.960           YBL016W FUS3    6287      
## 4  1.604           YKR093W PTR2   23012      
## 5  3.280           YHL021C AIM17    793      
## 6  5.191           YDL204W RTN2     418      
## 7  2.885           YML100W TSL1    1780      
## 8  1.124           YFL014W HSP12   9509      
## 9  3.862           YER185W PUG1     813      
## 10 1.013           YOR096W RPS7A  72660      
## ...
## 511 of 4875 non-zero standard deviation explained at FDR 0.05
## Prior df 21.2

4.4 Examine individual genes

Having discovered genes with differential tail length, let’s look at some genes in detail.

view_gene <- function(id) {
    gene <- rowData(wei)[id,"gene"]
    if (is.na(gene)) gene <- ""
    tails <- weitrix_x(cal)[id,]
    std_errs <- weitrix_weights(cal)[id,] ^ -0.5
    ggplot(samples) +
        aes(x=time,color=strain,group=strain, 
            y=tails, ymin=tails-std_errs, ymax=tails+std_errs) +
        geom_errorbar(width=0.2) + 
        geom_hline(yintercept=0) + 
        geom_line() + 
        geom_point(aes(size=tail_count[id,])) +
        labs(x="Time", y="Tail length", size="Read count", title=paste(id,gene)) +
        theme(axis.text.x=element_text(angle=90, hjust=1, vjust=0.5))
}

caption <- plot_annotation(
    caption="Error bars show +/- one standard error of measurement.")

# Top confident differences between WT and deltaSet1
view_gene("YDR170W-A") +
view_gene("YIL015W") +
view_gene("YAR009C") +
view_gene("YJR027W/YJR026W") +
caption

# Top confident changes over time
view_gene("YNL036W") +
view_gene("YBL097W") +
view_gene("YBL016W") +
view_gene("YKR093W") +
caption

5 Exploratory analysis: overdispersed genes

Genes with high dispersion (weighted residual variance) may be of biological interest. Here we examine dispersion relative to a simple model with only an intercept term. When the dispersion is greater than 1, there is variation in excess of that expected from our calibrated weights. The function weitrix_dispersions can be used to calculate dispersions.

To make this a bit more concrete, we can estimate how much extra variation there is per observation not explained by the model. The function weitrix_sd_confects provides this, and further provides a confident lower bound on this excess with a multiple testing correction. The “effect” column in the output is excess variation, and the “confect” column is a confident lower bound on this. Results are sorted by confect. These effects are in the same units as the observations themselves. They can be interpreted as the standard deviation if there was no observational error.

confects <- weitrix_sd_confects(cal, ~1)
confects
## $table
##    confect effect row_mean typical_obs_err dispersion n_present df fdr_zero 
## 1  4.714   7.857  45.91    3.092            7.456     20        19 0.000e+00
## 2  4.499   9.792  31.90    5.157            4.605     20        19 3.869e-09
## 3  4.354   6.001  29.37    1.761           12.608     20        19 0.000e+00
## 4  4.274   5.624  38.24    1.486           15.325     20        19 0.000e+00
## 5  4.274   5.910  30.67    1.804           11.739     20        19 0.000e+00
## 6  4.172   7.278  26.52    3.258            5.989     19        18 5.567e-13
## 7  3.904   4.999  32.85    1.243           17.182     20        19 0.000e+00
## 8  3.830   6.396  36.33    2.826            6.123     20        19 4.163e-14
## 9  3.739   5.754  30.83    2.267            7.443     20        19 0.000e+00
## 10 3.730   4.938  29.33    1.398           13.471     20        19 0.000e+00
##    name              gene   total_reads
## 1  YBL097W           BRN1    1680      
## 2  YDL204W           RTN2     418      
## 3  YNL036W           NCE103  5712      
## 4  YKR093W           PTR2   23012      
## 5  YBL016W           FUS3    6287      
## 6  YIL082W-A/YIL082W <NA>     842      
## 7  YDR461W           MFA1   83042      
## 8  YML100W           TSL1    1780      
## 9  YMR105C           PGM2    2616      
## 10 YCL042W/YCL040W   <NA>   12370      
## ...
## 745 of 4875 non-zero excess standard deviation at FDR 0.05

## Warning: Removed 1 row containing missing values (`geom_line()`).
## Warning: Removed 1 rows containing missing values (`geom_point()`).

The genes discovered tend to be changing over time. If we use a model that accounts for time, differences between the two strains will be emphasized instead.

confects2 <- weitrix_sd_confects(cal, ~time)
confects2
## $table
##    confect effect row_mean typical_obs_err dispersion n_present df fdr_zero 
## 1  3.018   5.094  20.61    1.516           12.299     20        10 0.000e+00
## 2  2.289   3.933  32.85    1.243           11.018     20        10 0.000e+00
## 3  2.259   3.571  18.35    1.022           13.214     20        10 0.000e+00
## 4  2.002   4.590  29.08    1.974            6.403     20        10 4.325e-07
## 5  1.905   3.995  26.23    1.631            7.001     20        10 5.374e-08
## 6  1.639   3.773  28.75    1.665            6.135     20        10 1.089e-06
## 7  1.531   3.173  31.76    1.309            6.877     20        10 7.457e-08
## 8  1.528   3.514  34.39    1.576            5.971     20        10 2.003e-06
## 9  1.209   2.616  25.12    1.133            6.329     20        10 5.250e-07
## 10 1.175   4.000  40.16    2.166            4.410     20        10 5.930e-04
##    name      gene total_reads
## 1  YDR476C   <NA>  4196      
## 2  YDR461W   MFA1 83042      
## 3  YNL208W   <NA> 23220      
## 4  YIL015W   BAR1  3898      
## 5  YDR170W-A <NA>  4832      
## 6  YKL128C   PMU1  5443      
## 7  YBR009C   HHF1 33533      
## 8  YDR224C   HTB1 13374      
## 9  YMR295C   <NA> 20878      
## 10 YOL092W   YPQ1  4661      
## ...
## 89 of 4875 non-zero excess standard deviation at FDR 0.05

6 Exploratory analysis: components of variation

The test we’ve performed was somewhat unsatisfactory. Due to the design of the experiment it’s difficul to specify differential tests that fully interrogate this dataset: the lack of replicates, and the difficult specifying apriori how tail length will change over time.

Perhaps we should let the data speak for itself.

Perhaps this is what we should have done first!

The weitrix package allows us to look for components of variation. We’ll try to explain the data with different numbers of components (from 1 to 6 components).

comp_seq <- weitrix_components_seq(cal, p=6)

weitrix_seq_screeplot shows how much additional variation in the data is explained as each further component is allowed. However the ultimate decision of how many components to examine is a matter of judgement.

components_seq_screeplot(comp_seq)

Looking at three components shows some of the major trends in this data-set.

comp <- comp_seq[[3]]

matrix_long(comp$col[,-1], row_info=samples, varnames=c("sample","component")) %>%
    ggplot(aes(x=time, y=value, color=strain, group=strain)) + 
    geom_hline(yintercept=0) + 
    geom_line() + 
    geom_point(alpha=0.75, size=3) + 
    facet_grid(component ~ .) +
    labs(title="Sample scores for each component", y="Sample score", x="Time", color="Strain")

We observe:

The tail lengths are approximated by comp$row %*% t(comp$col) where comp$col is an \(n_\text{sample} \times (p+1)\) matrix of scores (shown above), and comp$row is an \(n_\text{gene} \times (p+1)\) matrix of gene loadings, which we will now examine. (The \(+1\) is the intercept “component”, allowing each gene to have a different baseline tail length.)

Treat these results with caution. Confindence bounds take into account uncertainty in the loadings but not in the scores! What follows is best regarded as exploratory rather than a final result.

6.1 Gene loadings for C1: gradual lengthing over time

result_C1 <- weitrix_confects(cal, comp$col, coef="C1")
##    gene  loading confect total_reads
## 1  BRN1 4.679301   2.490        1680
## 2  FUS3 4.007695   2.408        6287
## 3  RTN2 6.188159   1.996         418
## 4  TBS1 3.387095   1.923        2872
## 5  PGM2 3.490045   1.800        2616
## 6  <NA> 3.400784   1.602        2342
## 7  <NA> 2.580025   1.580       12370
## 8  TSL1 3.098109   1.564        1780
## 9  GPA1 2.639603   1.560        5641
## 10 PTR2 2.538443   1.533       23012
## 1132 genes significantly non-zero at FDR 0.05

FUS3 is involved in yeast mating. We see here a poly(A) tail signature of yeast realizing there are not actually any \(\alpha\) cells around to mate with.

6.2 Gene loadings for C2: cell-cycle associated changes

result_C2 <- weitrix_confects(cal, comp$col, coef="C2")
##      gene   loading confect total_reads
## 1    RFA3  4.112870   1.909        3963
## 2    MSH6  5.279779   1.811         996
## 3    TOS6  4.704962   1.811        4024
## 4   CDC21  5.055944   1.803        1268
## 5  NCE103 -3.265461  -1.653        5712
## 6    GAS1  2.909671   1.638       49500
## 7    <NA>  3.339320   1.493       12356
## 8    SVS1  3.696601   1.329       11347
## 9    RNR1  3.372730   1.180        5659
## 10   HSL1  3.443047   1.139        3676
## 193 genes significantly non-zero at FDR 0.05

6.3 Gene loadings for C3: longer tails in set1 mutant

result_C3 <- weitrix_confects(cal, comp$col, coef="C3")

Given the mixture of signs for effects in C3, different genes are longer in different stages of the cell cycle. We see many genes to do with replication.

##      gene  loading confect total_reads
## 1    <NA> 4.154713   1.669        4196
## 2    BAR1 3.660681   1.506        3898
## 3    COX6 4.234550   1.141        1167
## 4    BAT1 2.417923   0.846        6868
## 5    POL4 4.154045   0.835         606
## 6    RPP0 1.838321   0.811       25545
## 7    RPL5 1.682070   0.761       81051
## 8    SSB2 1.735137   0.719       17238
## 9  RPL21B 1.817270   0.627       23159
## 10 RPS21A 1.596918   0.594       24574
## 336 genes significantly non-zero at FDR 0.05

7 Discussion

Looking back to our initial differential testing in light of these results, a reasonable refinement would be to omit “tpre” and “t0m”, considering only the samples that have settled into cell cycling.