Workshop Instructor Feedback #1452
Replies: 29 comments 20 replies
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Topics:
Audience: Fungal annotation people What did you like? Day 1:
Day 2:
Day 3:
What could be improved?
Day 2:
Day 3:
Originally posted by @erasche in #989 (comment) |
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Originally posted by @mblue9 in #989 (comment) @erasche great idea! Here's our workshop feedback from last week. Intro to Galaxy and RNA-seq Audience: Cancer biologists What did you like about this workshop?
What could be improved?
Any further comments or suggestions?
Myself and helper's (@rlupat) thoughts on improving General
Material Introduction
Reads to Counts
Counts to genes material
Genes to pathways
UI Feedback
Originally posted by @mblue9 in #989 (comment) |
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Intro to Galaxy Administration at GCC2019 Topics:
Helpers: @jmchilton Audience: Administrators (from beginning to advanced) and some developers What did you like about this workshop?
What could be improved?
Known bugs
Out of scope
Our thoughts on improving
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Galaxy Intro at MGC2019 at LUMC Topics:
Audience: Everyone from wet lab to bioinformatics students What did you like about this workshop? We informally collected feedback, all positive, useful for wet lab people even. Notes / Bugs
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Volcano plots with R, popup workshop at INAB|CERTH Topics
Audience: ca 10 bioinformaticians and programmers, all had some experience with R, a couple with Galaxy What did they like Bugs / TODOs
User Questions
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Galaxy Admin Training at the Barcelona Supercomputer Center Topics:
Audience: Everyone seemed super competent with command line already? (1 emacs user, 6 nano, 20+ vim). All galaxy admins. What did you like about this workshop? typos are my own. day 3
Cons:
day 1 Cons:
Pros:
Conclusions These will be discussed in #1809 but we have some ideas to improve the educational aspects. |
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Galaxy 101 for everyone The University of Melbourne, Australia - 24th & 25th September 2020 (Two sessions) Audience: Various science personnel - mostly post grads. Conducted online. Method: Online Likes: Really good general introduction to Galaxy and workflows. Lots of positive feedback from the students. Was very easy to teach. Cons: We were using Galaxy 20.05 and some of the screenshots and instructions are out of date 😞 . Not too big a deal as facilitators and trainers can easily point out differences. Conclusion: A really excellent tutorial. |
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De novo transcriptome reconstruction with RNA-Seq The University of Queensland, Australia - 13th October 2020 (one session). Method: Online (zoom) Pros: Well documented, uses popular tools (HiSAT2, StringTie, featureCounts). Cons: No explanation for advanced settings used with HiSAT2 esp for spliced alignment. It seems there is minor typo: HiSAT2 uses mm10, while in the Visualization step bamCoverage uses mm9 genome size. Also, Megakaryocyte_rep2 files have under 100k reads, while the remaining three samples have ~1M. Not sure if it is done on purpose, but very useful for QC. Very positive impression from the tutorial. |
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Reference-based RNA-Seq data analysis
General feedback (participants' perspective)
I will update this entry, if additional feedback is offered Instructor Feedback
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Workshop Name: Online data analysis for biologists (a.k.a Galaxy 101 for everyone) Date: 12 November 2020 URL: https://www.biocommons.org.au/events/galaxynov2020 Format: 3 hrs. Online via Zoom using a combination of lecture by the lead trainer and breakout rooms with facilitators where trainees worked through the exercises. Materials used: Galaxy 101 for everyone https://training.galaxyproject.org/training-material/topics/introduction/tutorials/galaxy-intro-101-everyone/tutorial.html Number of participants: 17 trainees, 5 trainers Audience: Biologists with no prior knowledge of Galaxy and no programming experience. What did you like about this workshop?
What could be improved?
Any further comments/suggestions
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@burkemlou be sure to check out the GTN-in-Galaxy feature, it addresses this issue, at least on EU :) https://training.galaxyproject.org/training-material/topics/contributing/tutorials/create-new-tutorial-content/tutorial.html#tool-links |
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Galaxy interactive tools, admin and dev hackathon
General feedback (participants' perspective)
Instructor Feedback
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Here's my workshop feedback from last week. Analysis of NextGen Sequencing Data in Galaxy Audience: Master Students and PhDs in Biology and Biochemistry. Using the Galaxy training material and the Galaxy Training Infrastructure as a service was an amazing experience. It is very easy to use and saves a lot of time setting up the course infrastructure. Pros:
Improvements:
Great resource! Highly recommended! |
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Workshop Name: Galaxy Introduction for Life Scientists Date: 27/04/2022 URL: https://www.sib.swiss/training/course/20220427_GALXY Format: 1 day. In person 🎉 Materials used: Crash test for the new version of Ref-based RNA-seq tutorial with collections and with the new choose your own tutorial. We did the STAR flavour. Number of participants: 14 trainees, 2 trainers (@hrhotz and @lldelisle) Audience: Biologists with no prior knowledge of Galaxy and no programming experience. What did you like about this workshop:
What could be improved?
Any further comments/suggestions
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just a few additional comments:
and of course a big Thank You to the Freiburg Galaxy team for offering TIaaS |
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I would like the sign for YOU NEED TO VERIFY YOUR LOGIN to be 100x bigger as this throws off initial students for AGES |
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Hello galaxy team, |
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Workshop Name: Molecular biology and genetics of the lepidoptera 2022 Date: 25/08/2022 URL: https://lepidoptera-2022.workshop.inrae.fr/ Format: 3h Materials used: Number of participants: ~20 trainees, 2 trainers (@stephanierobin and @abretaud), 2 helpers Audience: Biologists with minimal knowledge of Galaxy and no programming experience. What did you like about this workshop:
What could be improved?
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Hi Galaxy team, this is to let you know that I have started reproducing one of your variant calling tutorials using the command line tools. The first episode can be found here. I hope this helps others in the community. |
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Might be helpful if there was some automation associated with tutorials & tool versions for whenever there is a tool update to ping that the tutorial needs updating? Or like, 'this tutorial workflow hasn't been updated in a year' ping? |
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You know how you have all the cool icons etc. in the header of each tutorial, and/or the cool 'hands-on' sections, etc.? I was wondering about something like that but for input / answer key histories. I've had a number of instances of data import from Zenodo being slow and been saved by having either answer key histories or inputs, and it would be nice to have it distinguished from the main text a bit more because I inevitably have to point it out when people complain the import is taking forever and I ask if they tried the history import. |
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I put this somewhere before but cannot find it (sorry) but it's come up again in discussion with @hrukkudyr how it would be super helpful to have 'locked' histories, i.e. histories that we share for people to import because Zenodo is slow and/or we want them to see the answer key history. It's too easy to accidentally change them during analysis when you want to keep a few 'protected' for training purposes. |
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Hello,
Thank you for reaching out. I wanted to inform you that I am currently on paternity leave from the 15th of August until the 25th of September. During this period, I will not be available to respond to emails or attend to work-related matters.
I appreciate your understanding and patience during this special time for my family. I will respond to your email as soon as possible upon my return.
best regards,
Uwe
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Workshop Name: Learn how to analyze your sequencing data in few clicks Date: 26/10/2023 Format: 1 day and a half Announcement: During this training you will learn how to use Galaxy using a public Galaxy server. You will be able to retrieve public data, launch workflows in a few clicks and we will perform a full RNA-seq analysis as an example of a step-by-step in depth analysis. Materials used: Number of participants: 16 trainees, 2 trainers (@lldelisle and @hrhotz) Audience: Biologists from EPFL (where @lldelisle is working) with no knowledge of Galaxy and no programming experience. Global feedback from the trainers:
Global feedback from the trainees: Question to the trainees: What was one (or more) useful thing(s) that you learned during the workshop?
Question to the trainees: Did it make sense to build the workshop around a particular topic, i.e.: RNA-Seq?
Improvements for next time:
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Workshop: RNA-seq analysis: reads to differential expression Training materials: Day 2: RNA-seq counts to differential expression Length: 2x 3.5hr session over 10 and 11 September 2024 Format: Online via Zoom Number of participants: 35, life science researchers who are new to RNAseq analysis. They have data but have not analysed it themselves before. Feedback: The materials give great step by step instructions on executing the analysis steps in Galaxy. For future versions we plan to add more context about the overall process of RNAseq analysis, the purpose of each step and how this relates to the biological context. Most participants were very unfamiliar with the process and how it works. We had many questions about the why of the process for example, What is an adapter why do you need to remove them? Why is quality control important? How would these plots look if I was working on .....? We had problems uploading the data from Zenodo for the reads to counts part. We had to stagger running this job (5 people at a time) as when all 35 people tried to do it together the job repeatedly failed. I think this is a problem on the Zenodo end rather than with Galaxy. This made for a rocky start to the workshop but we got there in the end! Maria @mblue9 , Belinda and Harriet - you might want to change this step of the tutorial or at least add a note as I think this will be a common problem for anyone running this in a workshop setting. All in all, the workshop went well and 35 people now know more about RNAseq in Galaxy. Thanks for making the materials available via the GTN. |
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The workshop feedbacks are getting buried a bit in the tutorial feedback due to volume, so I'm separating those out into this new
issuediscussion :) Feel free to share your feedback from your workshop here, hopefully we can use this data to help identify common "papercuts" that new users are experiencing across workshops.Beta Was this translation helpful? Give feedback.
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