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CohortFinder


Intelligent data partitioning using quality control metrics

Purpose


Batch effects (BE) (e.g., scanner, stain variances), are systematic technical differences in data creation unrelated to biological variation. BEs have been shown to negatively impact machine learning (ML) model generalizability. Since they can result in the worst case when partioning patients into training/validation set, where patients in training set come from totally different BE groups from those in validation set. The purpose of the CohortFinder is to provide an intelligent data partition strategy trying to avoid the worst case situation without any manual effort.

CohortFinder has the following functionality:

  1. Cluster patients into different BE groups using quality control metrics
  2. Partition patients into training/validation set, making sure the patients in training or validation set come from all the BE groups

This tool can increase the performance and generalizability of machine learning model.

Requirements


Tested with Python 3.8.18 and 3.9.18

Requires:

  1. Python
  2. pip

And the following python packages:

  1. matplotlib

  2. numpy

  3. opencv-python-headless

  4. scikit-learn

  5. scipy

  6. umap

  7. pandas

Installation

1. Clone the CohortFinder github repository

git clone https://github.com/choosehappy/CohortFinder.git

2. (optional) Create a virtual environment

A python virtual environment (https://docs.python.org/3/library/venv.html) is the recommended dependency manager for CohortFinder.

cd CohortFinder
python3 -m venv cf_env
source cf_env/bin/activate

3. Install CohortFinder as a python package

pip install .

Quality Control Metrics Generation

Please see Histoqc and MRQy, these are 2 open-source quality control tools for digital pathology slides and imaging data. We use the quality control metrics it generates.

Basic Usage


The parameters CohortFinder used are as below:

python3 -m cohortfinder --help
usage: __main__.py [-h] [-c COLS] [-l LABELCOLUMN] [-s SITECOLUMN] [-p PATIENTIDCOLUMN] [-t TESTPERCENT] [-b] [-y] [-r RANDOMSEED] [-q] [-n NCLUSTERS]
                   resultsfilepath

Split histoqc/mrqy tsv into training and testing

positional arguments:
  resultsfilepath       The full path to the HistoQC/MRQy output file. This argument is required.

options:
  -h, --help            show this help message and exit
  -c COLS, --cols COLS  columns to use for clustering, comma seperated
  -l LABELCOLUMN, --labelcolumn LABELCOLUMN
                        column name associated with a 0,1 label
  -s SITECOLUMN, --sitecolumn SITECOLUMN
                        column name associated with site variable
  -p PATIENTIDCOLUMN, --patientidcolumn PATIENTIDCOLUMN
                        column name associated with patient id, ensuring slides are grouped
  -t TESTPERCENT, --testpercent TESTPERCENT
  -b, --batcheffectsitetest
  -y, --batcheffectlabeltest
  -r RANDOMSEED, --randomseed RANDOMSEED, for reproducing the same results for UMAP, k-means and data partitioning
  -q, --disable_save    Run silently, do not save any files.
  -d, --quality_control_tool Which quality tool is used here: HistoQC or MRQy (--histoqc/ --mrqy)
  -n NCLUSTERS, --nclusters NCLUSTERS
                        Number of clusters to attempt to divide data into before splitting into cohorts, default -1 of negative 1 makes best guess

Example run command:

python3 -m cohortfinder -n 4 -t 0.3 "/full/path/to/your/results.tsv"

Replace the filepath with a real file path, for example, we upload some sample data into the path "/test/histoqc_outdir/". You can do a quick test by using the following command

python3 -m cohortfinder -n 3 -t 0.3 -r 200  "/cohortfinder/test/histoqc_outdir/results.tsv"

Parameter meaning :

HistoQC

-c: metrics calculated by HistoQC we used for batch effect group generation, the default metrics are:
"mpp_x,mpp_y,michelson_contrast,rms_contrast,grayscale_brightness,chan1_brightness,chan2_brightness,chan3_brightness,chan1_brightness_YUV,chan2_brightness_YUV,chan3_brightness_YUV"

This is the description of the metrics used to identify the batch effects in our previous work, as they quantify chromatic artifacts imparted during the staining and cutting of the tissue samples steps conducted at individual laboratories before central scanning. And you can also try other metrics if they have some influence during the scanning or the staining process for your slides.

Quality control metric Description
Mpp_x Microns per pixel in the X dimension at base magnification
Mpp_y Microns per pixel in the Y dimension at base magnification
Michelson_constrast Measurement of image contrast defined by luminance difference over average luminance
Rms_contrast Root mean square (RMS) contrast, defined as the standard deviation of the pixel intensities across the pixels of interests
Grayscale_brightness Mean pixel intensity of the image after converting the image to grayscale
Chan1_brightness Mean pixel intensity of the red color channel of the image
Chan2_brightness Mean pixel intensity of the green color channel of the image
Chan3_brightness Mean pixel intensity of the blue color channel of the image
Chan1_brightness_YUV Mean channel brightness of red color channel of image after converting to YUV color space
Chan2_brightness_YUV Mean channel brightness of green color channel of image after converting to YUV color space
Chan3_brightness_YUV Mean channel brightness of blue color channel of image after converting to YUV color space

MRQy

-c: metrics calculated by MRQy we used for batch effect group generation, the default metrics are:
"MEAN,RNG,VAR,CV,CPP,PSNR,SNR1,SNR2,SNR3,SNR4,CNR,CVP,CJV,EFC,FBER"
Quality control metric Description
MEAN Mean of the foreground
RNG Range of the foreground
VAR Variance of the foreground
CV Coefficient of variation of the foreground for shadowing and inhomogeneity artifacts
CPP Contrast per pixel: mean of the foreground filtered by a 3×3 2D Laplacian kernel for shadowing artifacts
PSNR Peak signal to noise ratio of the foreground
SNR1 Foreground standard deviation (SD) divided by background SD
SNR2 Mean of the foreground patch divided by background SD
SNR3 Foreground patch SD divided by the centered foreground patch SD
SNR4 Mean of the foreground patch divided by mean of the background patch
CNR Contrast to noise ratio for shadowing and noise artifacts
CVP Coefficient of variation of the foreground patch for shading artifacts: foreground patch SD divided by foreground patch mean
CJV Coefficient of joint variation between the foreground and background for aliasing and inhomogeneity artifacts
EFC Entropy focus criterion for motion artifacts
FBER Foreground-background energy ratio for ringing artifacts

CohortFinder Output File Structure

Once you run the CohortFinder, you will get a cohortfinder result file called 'results_cohortfinder.tsv'. You will see two columns, one is called 'groupid', and the other is called 'testind', the testind == 1 represents the patients is partitioned into testing set and testind == 0 represents the patient is partitioned into the training set. You can simply use that patient partitioning results to set up the training set and test/val set for your machine learning model!

CohortFinder produces the following ouput file structure:

outputdir/ (default is histoqc/mrqy output directory)
    ... (histoqc/mrqy output, including results.tsv)
    cohortfinder_output_DATE_TIME/
        results_cohortfinder.tsv
        cohortfinder.log
        plots/
            embed.png
            embed_split.png
            embed_by_label.png (conditional)
            embed_by_site.png (conditional)
            group_0.png
            ...
            group_N.png
            allgroups.png

Outputs of CohortFinder

1. Result file and running log

The results_cohortfinder.tsv has four more columns than the histoqc/mrqy results.tsv file:

  1. groupid: the batch effect group assigned to the patient by cohortfinder.
  2. testind: the testing/training set assignment, where "1" patients were assigned to the testing set and "0" patients were assigned to the training set.
  3. embed_x: the UMAP embedding x coordinates.
  4. embed_y: the UMAP embedding y coordinates.

2. Embedding plots

Each point represents a patient and different colors represent different batch effect groups

embed

3. Patient partition plot

'x' represents the patients were split into training set and '+' means the patients were partitioned into testing set. You can also find the patients information detail in the results_cohortfinder.tsv file.

embed_split

4. The visual cluster results

embed_split

5. BE score

We also introduce three clustering metrics: the silhouette coefficient, the Davies-Bouldin index, and the Calinski-Harabasz index as BE scores. Here are the description of these 3 measurements. The measurements can be found in both cohortfinder tsv file and log file. Better score represents the cohort has severe batch-effect.

Quality control metric Description
Silhouette Coefficient(mean Silhouette Coefficient over all samples) Measures how similar an object is to its own cluster compared to other clusters. The value ranges from -1 to 1. A high value indicates appropriate clustering.
Davies-Bouldin index Measures how similar an object is to its own cluster compared to other clusters. The value ranges from -1 to 1. A high value indicates appropriate clustering.
Calinski-Harabasz index 1. Between-Cluster Dispersion: It measures how far the clusters are from each other. For good clustering, this should be as large as possible. 2.Within-Cluster Dispersion: It measures how compact the clusters are internally. For good clustering, this should be as small as possible.

Citation


Please use below to cite this paper if you find this repository useful or if you use the software shared here in your research.

  @misc{fan2023cohortfinder,
      title={CohortFinder: an open-source tool for data-driven partitioning of biomedical image cohorts to yield robust machine learning models}, 
      author={Fan Fan and Georgia Martinez and Thomas Desilvio and John Shin and Yijiang Chen and Bangchen Wang and Takaya Ozeki and Maxime W. Lafarge and Viktor H. Koelzer and Laura Barisoni and Anant Madabhushi and Satish E. Viswanath and Andrew Janowczyk},
      year={2023},
      eprint={2307.08673},
      archivePrefix={arXiv},
      primaryClass={cs.LG}
}

CohortFinder Paper link

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