Comparison of RNAi and small-molecule screens
Library design
Transfection
Kinetics and mechanism of RNAi action
Number and quality of controls
RNAi screening analysis workflow
Step 1: data triage
Step 2: normalization
Fraction or percentage of control
common approach
division each sample value by the mean of the control (either positive or negative)
requires a large number of controls to provide adequate estimation of their mean
sensitive to outliers
Fraction or percent of samples
common approach
the mean of samples on the plate may be substituted for the means of the controls
reduce the need for large numbers of controls
exacerbate the issue of nonrobustness
cannot incorporate information on the degree of variation in the sample data
z score and robust z score
z score: the number of standard deviations from the mean
frequently used in RNAi screening
incorporate information on the degree of variation in the sample data
depends on the use of samples as de facto negative controls
z score is sensitive to outliers-> robust z score, substitutes the outlier-insensitive median and median absolute deviation for mean and standard deviation in the z-score calculation
B score
for within-plate systematic effects
applied to remove row, column or well effects by iterative application of the Tukey median polish algorism
relatively robust to outliers
essentially uses the samples as negative controls
cellHT2 package in BioConductor bioinformatics software
Step 3: calculation of quality metrics
Z’ or Z factor
The most common quality metrics for RNAi and small-molecule screens
Z’ factor is often used during assay optimization (based on controls)
Z factor may be used to assess performance of the screen on actual samples
Strictly standardized mean difference (SSMD)
developed for use with RNAi screening
more rigorous than Z factor
the ratio between the difference of the means and the standard deviation of the difference between two populations
In one case, accurately captured the clear difference between the high and low populations, which is not detected by Z’ factor
Receiver operating characteristic curves (ROC)
used as quality metric in microarray transcriptomics
provides quick and intuitive understanding of dynamic ranges
multiple thresholds for defining positives and the resulting trade-offs between sensitivity and specificity can easily be investigated by plotting multiple ROC curve
used to compare validation performance of hits generated from differently normalized RNAi data
Step 4: hit identification
Median ±k median absolute deviation (MAD)
an improvement of mean ±k standard deviation approach
identify both strong and weak hits while controlling false positives
robust to outliers and to identify weak hits in RNAi data effectively
generate fewer false negatives than mean ±kstandard deviation
very easy to calculate
Multiple t-tests
simple to implement and understand, but requires three or more replicates of each condition
If a high false positive rate cannot be tolerated, it is imperative to apply multiple-comparison corrections to the resulting P-values of each individual test, resulting sensitive to outlier
Quartile-based selection
for the unsymmetrical data distribution
set upper and lower hits selection thresholds based on number of interquartile ranges above or below the first and third quartiles of the data
identify both strong and weak hits while controlling false positives
easy to calculate, but has not been general in RNAi screening (MAD is more common)
SSMD for hit identification
calculating the SSMD limits for hit selection based on the desired false positive rate, false negative rate or both
requires many negative controls
not calculated by standard analysis packages
Redundant siRNA activity (RSA)
integrate information about multiple RNAi reagents tested for each gene
ranks silencing reagents according to experimental effect and assigns a P-value to all reagents for single gene based on whether the reagents for that gene are distributed significantly higher in the rankings than would be expected by chance
be able to provide P-value for gene hits without sacrificing robustness
have higher rates of reconfirmation than those of identified with conventional methods
Although RSA is not included in common analysis software packages, ist developers have made available implementations in C# (for Windows), R and Perl
Rank product
originally developed for use with microarray data
The premise of the rank-product approach is that a consistent hit should be highly ranked in each independent biological replicate set.
provides P-values for potential hits without requiring the assumption of an underlying probability distribution
requires substantial computation and several replicates per screen to work
similar to RSA, but it does not depend on the use of multiple different RNAi reagents per gene
available as part of RNAither package in BioConductor
Bayesian models
To seek explicit estimated probabilities that a given siRNA has no effect, and inhibition effect or an activation effect
2 models are reported in 2008
simpler model; using only the negative controls to describe the posterior distribution of the ne true mean value for sample given the observed data value
more complex model; a posterior distribution that assumes the availability of data from both positive-inhibition and positive activation controls as well as negative controls
Both model provide the means to calculate the false discovery rate associated with any given hit threshold, but are usable only on screens without replicates
incorporates both plate-wide and experiment-wide information as well as information from both negative controls and the assumed de facto negative samples
simpler Bayesian model is followed by plate-wide MAD
not yet available in common software
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