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Genomic Data Processing - Data Eligibility Criteria (v-1.0)

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The NF-OSI is piloting a new initiative to uniformly process genomic and transcriptomic data that is shared on the NF Data Portal. The uniformly processed data will be shared on the NF Data Portal and will also be used to support the use of data from the NF Data Portal in other data analysis/exploration platforms. 

The processing of high dimensional genomic and transcriptomic data will be done using standardized data processing pipelines.

Thanks to the generosity of the NF-OSI funders, a subset of the NF Data Portal data is currently eligible for reprocessing as part of this initiative. If you have a dataset that you have shared on the NF Data Portal and would like to utilize the NF-OSI Processing pipelines, please reach out to us at nf-osi@sagebionetworks.org. We would be happy to assist you in a case-by-case basis.

Read the checklist below to learn more about which data are currently eligible for reprocessing.  

Studies in the current scope of this initiative:

All studies funded by the Neurofibromatosis Therapeutic Acceleration Program that uploaded data within the duration 2018 to 2023.

Data Types in the scope of processing:

  • Whole Exome Sequencing

  • Whole Genome Sequencing

  • Bulk RNA Sequencing

  • Single cell RNA sequencing

Eligibility criteria for data files to be staged for processing:

Required annotations for RNA Sequencing

Annotation term

Additional Details

1

fileFormat

Accepted file formats include "fastq", "bam", and "cram". If provided raw data are “bam” or “cram” format, only files that have not undergone any additional filtering (i.e. retains unmapped reads, have not been trimmed, etc) will be eligible for processing.

2

individualID

Individual IDs are necessary to create the sample sheets.

3

specimenID

specimen IDs are necessary to interpret the analysis.

4

Assay

Choose between Bulk RNA Seq or Single Cell RNA Seq.

5

Species

The corresponding genome requires knowledge of the species.

6

libraryPreparationMethod

This refers to the name of the library preparation, such as KAPA Hyper PCR 3.

7

Platform

This refers to the name of the platform used, for example, illumina.

8

readPair

Specify whether the read pair is 1 or 2.

9

specimenPreparationMethod

Minimize RNA degradation with methods such as flash freezing or RNALater. FFPE is not recommended.

10

tumorType

If the tissue is normal, indicate "not applicable." Otherwise, specify the tumor type.

11

isStranded*

This answer should be either "yes" or "no."

12

readPairOrientation*

Indicate the read pair orientation, such as forward or reverse.

* optional but recommended


Required annotations for Whole Genome Sequencing

Annotation term

Additional Details

1

fileFormat

Accepted file formats include "fastq", "bam", and "cram". If provided raw data are “bam” or “cram” format, only files that have not undergone any additional filtering (i.e. retains unmapped reads, have not been trimmed, etc) will be eligible for processing.

2

individualID

Individual IDs are necessary to create the sample sheets.

3

specimenID

specimen IDs are necessary to interpret the analysis.

4

Assay

Choose between Bulk RNA Seq or Single Cell RNA Seq.

5

Species

The corresponding genome requires knowledge of the species.

6

libraryPreparationMethod

This refers to the name of the library preparation, such as KAPA Hyper PCR 3.

7

Platform

This refers to the name of the platform used, for example, illumina.

8

readPair

Specify whether the read pair is 1 or 2.

9

specimenPreparationMethod

Minimize RNA degradation with methods such as flash freezing or RNALater. FFPE is not recommended.

10

tumorType

If the tissue is normal, indicate "not applicable." Otherwise, specify the tumor type. NOTE: Files from samples lacking tumor-normal pairs will not be eligible for Somatic variant calls or for microsatellite instability processing.

11

isStranded*

This answer should be either "yes" or "no."

12

readPairOrientation*

Indicate the read pair orientation, such as forward or reverse.

* optional but recommended


Required annotations for Whole Exome Sequencing

Annotation term

Additional Details

1

fileFormat

Accepted file formats include "fastq", "bam", and "cram". If provided raw data are “bam” or “cram” format, only files that have not undergone any additional filtering (i.e. retains unmapped reads, have not been trimmed, etc) will be eligible for processing. Note: WES files are not eligible for variant calling if BED file is not available

2

individualID

Individual IDs are necessary to create the sample sheets.

3

specimenID

specimen IDs are necessary to interpret the analysis.

4

Assay

Choose between Bulk RNA Seq or Single Cell RNA Seq.

5

Species

The corresponding genome requires knowledge of the species.

6

libraryPreparationMethod

This refers to the name of the library preparation, such as KAPA Hyper PCR 3.

7

Platform

This refers to the name of the platform used, for example, illumina.

8

readPair

Specify whether the read pair is 1 or 2.

9

specimenPreparationMethod

Minimize RNA degradation with methods such as flash freezing or RNALater. FFPE is not recommended.

10

tumorType

If the tissue is normal, indicate "not applicable." Otherwise, specify the tumor type. NOTE: Files from samples lacking tumor-normal pairs will not be eligible for Somatic variant calls or for microsatellite instability processing.

11

isStranded*

This answer should be either "yes" or "no."

12

readPairOrientation*

Indicate the read pair orientation, such as forward or reverse.

* optional but recommended

Availability of processing workflows:

The table below shows the availability of processing workflows for different data files generated through various ‘omics assays. 

✅ means the workflow is Available for the data files 

❌ means the workflow is available for these kind of data files but the NF-OSI will not provide this processing. This decision follows from the recommendation of scientists and engineers at Sage who have worked with these data modalities and have noted various problems in interpretation of processed data from these workflows during downstream analysis. 

NA means the workflow is not applicable for these data files

Assay

Germline SNV

Somatic SNV

Copy Number Variation (CNV)

Structural variants (SV)

Microsatellite Instability (MSI)

Raw counts

WES

NA

WGS

NA

Bulk RNAseq

NA

NA

NA

NA

NA

Single Cell RNAseq

NA

NA

NA

NA

NA

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