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--- |
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license: cc-by-nc-sa-4.0 |
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language: |
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- en |
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tags: |
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- Genomics |
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- Benchmarks |
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- Language Models |
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- DNA |
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pretty_name: Genomics Long-Range Benchmark |
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viewer: false |
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--- |
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## Summary |
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The motivation of the genomics long-range benchmark (LRB) is to compile a set of |
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biologically relevant genomic tasks requiring long-range dependencies which will act as a robust evaluation tool for genomic language models. |
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While serving as a strong basis of evaluation, the benchmark must also be efficient and user-friendly. |
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To achieve this we strike a balance between task complexity and computational cost through strategic decisions, such as down-sampling or combining datasets. |
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## Benchmark Tasks |
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The Genomics LRB is a collection of nine tasks which can be loaded by passing in the |
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corresponding `task_name` into the `load_dataset` function. All of the following datasets |
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allow the user to specify an arbitrarily long sequence length, giving more context |
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to the task, by passing the `sequence_length` kwarg to `load_dataset`. Additional task |
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specific kwargs, if applicable, are mentioned in the sections below.<br> |
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*Note that as you increase the context length to very large numbers you may start to reduce the size of the dataset since a large context size may |
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cause indexing outside the boundaries of chromosomes. |
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| Task | `task_name` | Sample Output | ML Task Type | # Outputs | # Train Seqs | # Test Seqs | Data Source | |
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|-------|-------------|-------------------------------------------------------------------------------------------|-------------------------|-------------|--------------|----------- |----------- | |
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| Variant Effect Causal eQTL | `variant_effect_causal_eqtl` | {ref sequence, alt sequence, label, tissue, chromosome,position, distance to nearest TSS} | SNP Classification | 1 | 88717 | 8846 | GTEx (via [Enformer](https://www.nature.com/articles/s41592-021-01252-x)) | |
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| Variant Effect Pathogenic ClinVar | `variant_effect_pathogenic_clinvar` | {ref sequence, alt sequence, label, chromosome, position} | SNP Classification | 1 | 38634 | 1018 | ClinVar, gnomAD (via [GPN-MSA](https://www.biorxiv.org/content/10.1101/2023.10.10.561776v1)) | |
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| Variant Effect Pathogenic OMIM | `variant_effect_pathogenic_omim` | {ref sequence, alt sequence, label,chromosome, position} | SNP Classification | 1 | - | 2321473 |OMIM, gnomAD (via [GPN-MSA](https://www.biorxiv.org/content/10.1101/2023.10.10.561776v1)) | |
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| CAGE Prediction | `cage_prediction` | {sequence, labels, chromosome,label_start_position,label_stop_position} | Binned Regression | 50 per bin | 33891 | 1922 | FANTOM5 (via [Basenji](https://journals.plos.org/ploscompbiol/article?id=10.1371/journal.pcbi.1008050)) | |
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| Bulk RNA Expression | `bulk_rna_expression` | {sequence, labels, chromosome,position} | Seq-wise Regression | 218 | 22827 | 990 | GTEx, FANTOM5 (via [ExPecto](https://www.nature.com/articles/s41588-018-0160-6)) | |
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| Chromatin Features Histone_Marks | `chromatin_features_histone_marks` | {sequence, labels,chromosome, position, label_start_position,label_stop_position} | Seq-wise Classification | 20 | 2203689 | 227456 | ENCODE, Roadmap Epigenomics (via [DeepSea](https://pubmed.ncbi.nlm.nih.gov/30013180/) | |
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| Chromatin Features DNA_Accessibility | `chromatin_features_dna_accessibility` | {sequence, labels,chromosome, position, label_start_position,label_stop_position} | Seq-wise Classification | 20 | 2203689 | 227456 | ENCODE, Roadmap Epigenomics (via [DeepSea](https://pubmed.ncbi.nlm.nih.gov/30013180/)) | |
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| Regulatory Elements Promoter | `regulatory_element_promoter` | {sequence, label,chromosome, start, stop, label_start_position,label_stop_position} | Seq-wise Classification | 1| 953376 | 96240 | SCREEN | |
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| Regulatory Elements Enhancer | `regulatory_element_enhancer` | {sequence, label,chromosome, start, stop, label_start_position,label_stop_position} | Seq-wise Classification | 1| 1914575 | 192201 | SCREEN | |
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## Usage Example |
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```python |
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from datasets import load_dataset |
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# Use this parameter to download sequences of arbitrary length (see docs below for edge cases) |
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sequence_length=2048 |
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# One of: |
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# ["variant_effect_causal_eqtl","variant_effect_pathogenic_clinvar", |
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# "variant_effect_pathogenic_omim","cage_prediction", "bulk_rna_expression", |
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# "chromatin_features_histone_marks","chromatin_features_dna_accessibility", |
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# "regulatory_element_promoter","regulatory_element_enhancer"] |
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task_name = "variant_effect_causal_eqtl" |
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dataset = load_dataset( |
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"InstaDeepAI/genomics-long-range-benchmark", |
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task_name=task_name, |
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sequence_length=sequence_length, |
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) |
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``` |
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### 1. Variant Effect Causal eQTL |
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Predicting the effects of genetic variants, particularly expression quantitative trait loci (eQTLs), is essential for understanding the molecular basis of several diseases. |
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eQTLs are genomic loci that are associated with variations in mRNA expression levels among individuals. |
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By linking genetic variants to causal changes in mRNA expression, researchers can |
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uncover how certain variants contribute to disease development. |
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#### Source |
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Original data comes from GTEx. Processed data in the form of vcf files for positive |
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and negative variants across 49 different tissue types were obtained from the |
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[Enformer paper](https://www.nature.com/articles/s41592-021-01252-x) located [here](https://console.cloud.google.com/storage/browser/dm-enformer/data/gtex_fine/vcf?pageState=%28%22StorageObjectListTable%22:%28%22f%22:%22%255B%255D%22%29%29&prefix=&forceOnObjectsSortingFiltering=false). |
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Sequence data originates from the GRCh38 genome assembly. |
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#### Data Processing |
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Fine-mapped GTEx eQTLs originate from [Wang et al](https://www.nature.com/articles/s41467-021-23134-8), while the negative matched set of |
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variants comes from [Avsec et al](https://www.nature.com/articles/s41592-021-01252-x) |
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. The statistical fine-mapping tool SuSiE was used to label variants. |
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Variants from the fine-mapped eQTL set were selected and given positive labels if |
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their posterior inclusion probability was > 0.9, |
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as assigned by SuSiE. Variants from the matched negative set were given negative labels if their |
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posterior inclusion probability was < 0.01. |
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#### Task Structure |
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Type: Binary classification<br> |
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Task Args:<br> |
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`sequence_length`: an integer type, the desired final sequence length<br> |
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Input: a genomic nucleotide sequence centered on the SNP with the reference allele at the SNP location, a genomic nucleotide sequence centered on the SNP with the alternative allele at the SNP location, and tissue type<br> |
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Output: a binary value referring to whether the variant has a causal effect on gene |
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expression |
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#### Splits |
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Train: chromosomes 1-8, 11-22, X, Y<br> |
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Test: chromosomes 9,10 |
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--- |
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### 2. Variant Effect Pathogenic ClinVar |
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A coding variant refers to a genetic alteration that occurs within the protein-coding regions of the genome, also known as exons. |
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Such alterations can impact protein structure, function, stability, and interactions |
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with other molecules, ultimately influencing cellular processes and potentially contributing to the development of genetic diseases. |
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Predicting variant pathogenicity is crucial for guiding research into disease mechanisms and personalized treatment strategies, enhancing our ability to understand and manage genetic disorders effectively. |
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#### Source |
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Original data comes from ClinVar and gnomAD. However, we use processed data files |
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from the [GPN-MSA paper](https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10592768/) |
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located [here](https://huggingface.co/datasets/songlab/human_variants/blob/main/test.parquet). |
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Sequence data originates from the GRCh38 genome assembly. |
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#### Data Processing |
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Positive labels correspond to pathogenic variants originating from ClinVar whose review status was |
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described as having at least a single submitted record with a classification but without assertion criteria. |
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The negative set are variants that are defined as common from gnomAD. gnomAD version 3.1.2 was downloaded and filtered to variants with allele number of at least 25,000. Common |
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variants were defined as those with MAF > 5%. |
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#### Task Structure |
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Type: Binary classification<br> |
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Task Args:<br> |
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`sequence_length`: an integer type, the desired final sequence length<br> |
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Input: a genomic nucleotide sequence centered on the SNP with the reference allele at the SNP location, a genomic nucleotide sequence centered on the SNP with the alternative allele at the SNP location<br> |
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Output: a binary value referring to whether the variant is pathogenic or not |
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#### Splits |
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Train: chromosomes 1-7, 9-22, X, Y<br> |
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Test: chromosomes 8 |
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--- |
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### 3. Variant Effect Pathogenic OMIM |
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Predicting the effects of regulatory variants on pathogenicity is crucial for understanding disease mechanisms. |
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Elements that regulate gene expression are often located in non-coding regions, and variants in these areas can disrupt normal cellular function, leading to disease. |
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Accurate predictions can identify biomarkers and therapeutic targets, enhancing personalized medicine and genetic risk assessment. |
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#### Source |
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Original data comes from the Online Mendelian Inheritance in Man (OMIM) and gnomAD |
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databases. |
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However, we use processed data files from the |
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[GPN-MSA paper](https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10592768/) located [here]( |
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https://huggingface.co/datasets/songlab/omim/blob/main/test.parquet). |
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Sequence data originates from the GRCh38 genome assembly. |
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#### Data Processing |
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Positive labeled data originates from a curated set of pathogenic variants located |
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in the Online Mendelian Inheritance in Man (OMIM) catalog. The negative set is |
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composed of variants that are defined as common from gnomAD. gnomAD version 3.1.2 was downloaded and filtered to variants with |
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allele number of at least 25,000. Common variants were defined as those with minor allele frequency |
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(MAF) > 5%. |
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#### Task Structure |
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Type: Binary classification<br> |
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Task Args:<br> |
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`sequence_length`: an integer type, the desired final sequence length<br> |
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`subset`: a boolean type, whether to use the full dataset or a subset of the dataset (we provide this option as the full dataset has millions of samples) |
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Input: a genomic nucleotide sequence centered on the SNP with the reference allele at the SNP location, a genomic nucleotide sequence centered on the SNP with the alternative allele at the SNP location<br> |
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Output: a binary value referring to whether the variant is pathogenic or not |
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#### Splits |
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Test: all chromosomes |
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--- |
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### 4. CAGE Prediction |
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CAGE provides accurate high-throughput measurements of RNA expression by mapping TSSs at a nucleotide-level resolution. |
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This is vital for detailed mapping of TSSs, understanding gene regulation mechanisms, and obtaining quantitative expression data to study gene activity comprehensively. |
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#### Source |
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Original CAGE data comes from FANTOM5. We used processed labeled data obtained from |
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the [Basenji paper](https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5932613/) which |
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also used to train Enformer and is located [here](https://console.cloud.google.com/storage/browser/basenji_barnyard/data/human?pageState=%28%22StorageObjectListTable%22:%28%22f%22:%22%255B%255D%22%29%29&prefix=&forceOnObjectsSortingFiltering=false). |
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Sequence data originates from the GRCh38 genome assembly. |
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#### Data Processing |
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The original dataset from the Basenji paper includes labels for 638 CAGE total tracks over 896 bins (each bin corresponding to 128 base pairs) |
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totaling over ~70 GB. In the interest of dataset size and user-friendliness, only a |
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subset of the labels are selected. |
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From the 638 CAGE tracks, 50 of these tracks are selected with the following criteria: |
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1. Only select one cell line |
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2. Only keep mock treated and remove other treatments |
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3. Only select one donor |
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The [896 bins, 50 tracks] labels total in at ~7 GB. A description of the 50 included CAGE tracks can be found here `cage_prediction/label_mapping.csv`. |
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*Note the data in this repository for this task has not already been log(1+x) normalized. |
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#### Task Structure |
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Type: Multi-variable regression<br> |
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Because this task involves predicting expression levels for 128bp bins and there are 896 total bins in the dataset, there are in essence labels for 896 * 128 = 114,688 basepair sequences. If |
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you request a sequence length smaller than 114,688 bps than the labels will be subsetted. |
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Task Args:<br> |
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`sequence_length`: an integer type, the desired final sequence length, *must be a multiple of 128 given the binned nature of labels<br> |
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Input: a genomic nucleotide sequence<br> |
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Output: a variable length vector depending on the requested sequence length [requested_sequence_length / 128, 50] |
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#### Splits |
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Train/Test splits were maintained from Basenji and Enformer where randomly sampling was used to generate the splits. Note that for this dataset a validation set is also returned. In practice we merged the validation |
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set with the train set and use cross validation to select a new train and validation set from this combined set. |
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--- |
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### 5. Bulk RNA Expression |
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Gene expression involves the process by which information encoded in a gene directs the synthesis of a functional gene product, typically a protein, through transcription and translation. |
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Transcriptional regulation determines the amount of mRNA produced, which is then translated into proteins. Developing a model that can predict RNA expression levels solely from sequence |
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data is crucial for advancing our understanding of gene regulation, elucidating disease mechanisms, and identifying functional sequence variants. |
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#### Source |
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Original data comes from GTEx. We use processed data files from the [ExPecto paper](https://www.nature.com/articles/s41588-018-0160-6) found |
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[here](https://github.com/FunctionLab/ExPecto/tree/master/resources). Sequence data originates from the GRCh37/hg19 genome assembly. |
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#### Data Processing |
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The authors of ExPecto determined representative TSS for Pol II transcribed genes |
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based on quantification of CAGE reads from the FANTOM5 project. The specific procedure they used is as |
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follows, a CAGE peak was associated to a GENCODE gene if it was withing 1000 bps from a |
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GENCODE v24 annotated TSS. The most abundant CAGE peak for each gene was then selected |
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as the representative TSS. When no CAGE peak could be assigned to a gene, the annotated gene |
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start position was used as the representative TSS. We log(1 + x) normalized then standardized the |
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RNA-seq counts before training models. A list of names of tissues corresponding to |
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the labels can be found here: `bulk_rna_expression/label_mapping.csv`. *Note the |
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data in this repository for this task has already been log(1+x) normalized and |
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standardized to mean 0 and unit variance. |
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#### Task Structure |
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Type: Multi-variable regression<br> |
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Task Args:<br> |
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`sequence_length`: an integer type, the desired final sequence length<br> |
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Input: a genomic nucleotide sequence centered around the CAGE representative trancription start site<br> |
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Output: a 218 length vector of continuous values corresponding to the bulk RNA expression levels in 218 different tissue types |
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#### Splits |
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Train: chromosomes 1-7,9-22,X,Y<br> |
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Test: chromosome 8 |
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--- |
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### 6. Chromatin Features |
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Predicting chromatin features, such as histone marks and DNA accessibility, is crucial for understanding gene regulation, as these features indicate chromatin state and are essential for transcription activation. |
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#### Source |
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Original data used to generate labels for histone marks and DNase profiles comes from the ENCODE and Roadmap Epigenomics project. We used processed data files from the [Deep Sea paper](https://www.nature.com/articles/nmeth.3547) to build this dataset. |
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Sequence data originates from the GRCh37/hg19 genome assembly. |
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#### Data Processing |
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The authors of DeepSea processed the data by chunking the human genome |
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into 200 bp bins where for each bin labels were determined for hundreds of different chromatin |
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features. Only bins with at least one transcription factor binding event were |
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considered for the dataset. If the bin overlapped with a peak region of the specific |
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chromatin profile by more than half of the |
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sequence, a positive label was assigned. DNA sequences were obtained from the human reference |
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genome assembly GRCh37. To make the dataset more accessible, we randomly sub-sampled the |
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chromatin profiles from 125 to 20 tracks for the histones dataset and from 104 to 20 tracks for the |
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DNA accessibility dataset. |
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#### Task Structure |
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Type: Multi-label binary classification |
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Task Args:<br> |
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`sequence_length`: an integer type, the desired final sequence length<br> |
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`subset`: a boolean type, whether to use the full dataset or a subset of the dataset (we provide this option as the full dataset has millions of samples) |
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Input: a genomic nucleotide sequence centered on the 200 base pair bin that is associated with the labels<br> |
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Output: a vector of length 20 with binary entries |
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#### Splits |
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Train set: chromosomes 1-7,10-22<br> |
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Test set: chromosomes 8,9 |
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--- |
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### 7. Regulatory Elements |
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Cis-regulatory elements, such as promoters and enhancers, control the spatial and temporal expression of genes. |
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These elements are essential for understanding gene regulation mechanisms and how genetic variations can lead to differences in gene expression. |
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#### Source |
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Original data annotations to build labels came from the Search Candidate cis-Regulatory Elements by ENCODE project. Sequence data originates from the GRCh38 |
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genome assembly. |
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#### Data Processing |
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The data is processed as follows, we break the human |
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reference genome into 200 bp non-overlapping chunks. If the 200 bp chunk overlaps by at least 50% |
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or more with a contiguous region from the set of annotated cis-regulatory elements (promoters or |
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enhancers), we label them as positive, else the chunk is labeled as negative. The resulting dataset |
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was composed of ∼15M negative samples and ∼50k positive promoter samples and ∼1M positive |
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enhancer samples. We randomly sub-sampled the negative set to 1M samples, and kept |
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all positive |
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samples, to make this dataset more manageable in size. |
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#### Task Structure |
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Type: Binary classification |
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Task Args:<br> |
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`sequence_length`: an integer type, the desired final sequence length<br> |
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`subset`: a boolean type, whether to use the full dataset or a subset of the dataset (we provide this option as the full dataset has millions of samples) |
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Input: a genomic nucleotide sequence centered on the 200 base pair bin that is associated with the label<br> |
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Output: a single binary value |
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#### Splits |
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Train set: chromosomes 1-7,10-22<br> |
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Test set: chromosomes 8,9 |
