Lexogen Online FAQs
How do I analyze my QuantSeq FWD-UMI Sequencing Data?
- Matteo Carina (Unlicensed)
- Nathalie Durut
- Simona Ferraioli (Unlicensed)
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Lexogen Data Analysis Solution
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QuantSeq FWD-UMI data can be analyzed using our new web-based interactive platform, Kangooroo. QuantSeq kits are provided with a voucher code which can be used for the data analysis. If additional codes are needed, please contact sales@lexogen.com.
For further information about how to process your data, please visit our Webpage https://www.lexogen.com/lexogen-data-analysis-solutions/ and check out these online FAQs.
UMI-Tools
As an alternative to the data analysis solution offered by Lexogen, we recommend utilizing the publicly available UMI-Tools package available on GitHub here. Detailed documentation can be found in the ReadTheDocs. The following command line will extract the UMI sequence from the read while removing the adjacent 4 nt TATA spacer:
umi_tools extract --extract-method=regex --bc-pattern "(?P<umi_1>.{6})(?P<discard_1>.{4}).*" -L "/path/to/my_outputlog.txt" -I "/path/to/my_input.fastq.gz" -S "/path/to/my_output.fastq.gz"
After alignment, reads can be deduplicated with the following command:
umi_tools dedup -I example.bam --output-stats=deduplicated -S deduplicated.bamÂ
The deduplication method of UMI-Tools has been published here.
NOTE: The current implementation of this method can take some time and can consume significant memory. If you experience issues with run time or memory usage, please refer to these FAQs.
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If you would like to run the package in a less complex way, you can set the parameter:
"-method=unique"This will only collapse UMIs having identical sequences.
For further information contact us at support@lexogen.com.
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Have feedback for us or need more information? Send us a request or write to us at support@lexogen.com.