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Dram1.4rc #207
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…n print_database_locations with logging.info
…n get_gene_neighborhoods
The important thing to know is that I think the count should be per gene, not per genome. They are called internally in dram but they are genes. So if there is one gene in a genome with AA1_2;AA1_3 that is a count of one in the distillate, if there is another gene with say AA1_4;AA1_5;AA1_2 on another line of the annotations, then each AA1_2;AA1_3 and AA1_4;AA1_5;AA1_2 would count for 1 and AA1 would have a count of 2.
Change all FTP URLs to HTTP(s) to avoid firewall/ACL issues
Here is the release note for this release candidate. It is still a candidate and will not automatically update. This is the first release candidate of DRAM1.4.0. The 1.4.0 release has significant changes that could impact your research. Please review these changes and help us validate this release! Install / upgrade:In a few weeks DRAM will be upgraded in Bioconda and then can be upgraded like any Conda package. You will still be able to install DRAM1.3.5 with the traditional Conda method outlined in the README, but for early adoption you will need to use the method of install below. This method is also added in the README under Install Release Candidate. To install a potentially unstable release candidate of DRAM, use the set of commands below that are suitable to your situation. Note the comments within the code sections and there is a context in which commands must be used. If you already have a DRAM environment and want to upgrade:
To install the DRAM release candidate in a new Conda environment;
Change log:
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