Difference between revisions of "20th Discussion-6 Feb 2018"

Revision as of 09:26, 6 February 2018

How much training do you do?

2-3 full days modeled on software carpentry, done a few times, command line, RNA-seq
Simon Andrews, Babraham Institute
- huge amount of training, 50 courses a year, a day each
- one of their core functions
- internal / external / commercial venture
- 5 regular teachers
Matt Eldridge, Cambridge
- Also a large amount of training
- Part of a larger university program
- demand is massive, long waiting list
- perhaps have noticed routine analysis going down in volume
  - maybe that's fine, let routine stuff go and focus on harder analyses
How much? free?
- 50 pounds a day for postdocs, Phd students free
- 178 pounds a day with a "day rate"

Curriculum?

command line, common bioinfo tools
RNA-seq / ChIP-seq / application specific
someone suggested github / docker
Simon said they do
- statistics
- core skills - unix, perl/python, R
- RNA-seq / chIP-seq / methyl-seq
- "creating figures"
- gene set enrichment analysis
Goblet was mentioned
- but direct reuse is harder than it seems
Environments are tricky
- how do you ensure the same environment for everyone?
- amazon - but then dependent on network
- some people use docker - last part of course is getting things running on *your* laptop
- Use a script to check that everything is installed and ready to go

Nanopore

Who is doing it and what are your experiences?
Now they have a direct RNA sequencing kit
minoTour - realtime nanopore monitoring
Mark, UW Madison - quality of flowcells drops considerally, they run 32-36 hours
Nanopore is operator / library sensitive
air bubbles in flowcell can happen
EDTA will kill it
Minknow is the software from oxford nanopore, mac/linux/windows, downstream albacore
smaller flowcells are coming - running a smidgeon on a minion
minion_qc on github useful QC plots, minimap2 for alignment
epitome from ONT
WIMP - what's in my pot
how about base modifications?
- nanopolish can report methylated bases, but some question about accuracy. Paper in nature methods
- Simon mentioned trying to use it to assemble immunoglobulin, found nanopolish was over collapsing their reads

@@ Line 46: / Line 46: @@
 * Which tools have you found useful thus far for analysis?
 * Any particular quality control approaches you are using?
+Nanopore
+* Who is doing it and what are your experiences?
+* Now they have a direct RNA sequencing kit
+* minoTour - realtime nanopore monitoring
+* Mark, UW Madison - quality of flowcells drops considerally, they run 32-36 hours
+* Nanopore is operator / library sensitive
+* air bubbles in flowcell can happen
+* EDTA will kill it
+* Minknow is the software from oxford nanopore, mac/linux/windows, downstream albacore
+* smaller flowcells are coming - running a smidgeon on a minion
+* minion_qc on github useful QC plots, minimap2 for alignment
+* epitome from ONT
+* WIMP - what's in my pot
+* how about base modifications?
+** nanopolish can report methylated bases, but some question about accuracy. Paper in nature methods
+** Simon mentioned trying to use it to assemble immunoglobulin, found nanopolish was over collapsing their reads
 == Other New Protocols or Approaches? ==
 * Anything new happening at your institution that you would like to discuss?