/r/proteomics/

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  • built a peptide reference site because i was tired of pulling data from 6 different places every time i wanted to actually understand a compound
    by /u/Clinpep
    submitted by /u/Clinpep [link] [comments]
  • Expanding the human proteome with microproteins and peptideins
    by /u/Dwarvling
    Approximately 25% of 7200 noncoding open reading frames in humane genome encode detectable peptides of unknown function. submitted by /u/Dwarvling [link] [comments]
  • Why do proteomics journals have relatively low impact factors?
    by /u/MilkF5
    I have been working in proteomics for about 5 years. Recently, I had a discussion with my supervisor about why proteomics journals usually have relatively low impact factors. To be honest, I avoided submitting to these journals for years because of that. We usually preferred broader biomedical journals. But recently I changed my mind a bit. I submitted two papers to Proteomics and one to Journal of Proteome Research. Now I wonder if impact factor is a bit misleading in this field. Proteomics is very important, but many papers are technical, dataset-based, or useful mainly to a specialized audience. The […]
  • Question regarding C18 spin columns
    by /u/bluemooninvestor
    Hello everyone, I have been using Pierce Desalting Spin columns for peptide cleanup, and it required 300 uL of 50% ACN to elute. Now, I have to use the Pierce C18 columns. Despite both of them being small spin columns, the C18 column protocol says that only 20 uL of 70% ACN should be used for elution. My question is, isn't 20 uL a very small volume? Why is there such a huge difference in elution volume between the two spin columns (Desalting v C18 one)? Lastly, is there any general understanding in the proteomics community to use a larger […]
  • Is there anything genuinely new in bioinformatics for proteomics analysis?
    by /u/MilkF5
    I have been reading a lot of recent proteomics papers, especially LC-MS/MS quantitative proteomics studies, and I keep getting the impression that most downstream bioinformatics workflows are basically the same. A typical pipeline seems to be something like: preprocessing/filtering of protein or peptide abundance matrizes normalization, often VSN, median normalization, quantile normalization, etc. missing value imputation, usually MinProb, random forest, KNN, QRILC, or some variant differential abundance analysis with limma, MSstats, DEP, proDA, DEqMS, or now newer tools like limpa volcano plots heatmaps/PCA clustering, sometimes Mfuzz co-expression/module analysis, sometimes WGCNA ORA/GSEA/pathway enrichment STRING/Cytoscape protein-protein interaction networks And then the biological […]
  • TMT11 labelling efficiency issues?
    by /u/Capable_Vegetable293
    Is anyone experiencing issues with TMT11 labelling efficiency? I'm from a lab that has done TMT proteomics for many years and >99% labelling efficiency is standard for us. Over the past few weeks we’ve seen a drop to around 80% efficiency. We've changed everything we can think of on our end and are thinking it might be a manufactuing problem. submitted by /u/Capable_Vegetable293 [link] [comments]
  • PEAKS Software
    by /u/Proteo-Freak973
    Does anyone use PEAKS software by bioinformatics solutions for Proteomics data analysis? I am new to it and want to understand how you analyze the data and which parameters you mostly change and why? submitted by /u/Proteo-Freak973 [link] [comments]
  • Does anyone have a detailed workflow of how to anlayse pride proteomic datasets for re-analyses.
    by /u/HowlettXavier_522352
    Hi. I wanted to analyse some publicly available proteomic datasets to validate some of our own proteomic results. I thought of making use of the PRIDE proteomic database. I am having a slight confusion on how to go about it. If anyone has previously done the analyses, starting from download the dataset, processing if needed and analyses using RStudio, or anything like that…. Could someone who is free please help out Thanks you so much, really means a lot! submitted by /u/HowlettXavier_522352 [link] [comments]
  • Somascan vs OLink for CSF
    by /u/poly_cherry
    I am planning to go for the big panels – Somascan 11k or OLink Explore HT (~5.3k) for my CSF samples. Somascan's menu is more accessible and gives detailed QC metrics for all their proteins – and has a good hit rate of my proteins of interest. OLink is a bit more opaque about the performance of sepcific proteins. I am also leaning more towards Somascan as it is larger and offers it as a service and charges per sample (instead of plate). Apart from logistical advantages – why should anyone choose one over the other. Anyspecific downsides of somascan? […]
  • Why are there so many papers describing advanced proteomics techniques, but so few papers actually using them?
    by /u/bluemooninvestor
    Recently I have run into Lip-ms, and there are quite a few high impact papers describing the technique. But there are really few papers who have actually used it for doing science. I think it is the same for several other techniques like proximity-labelling MS, certain advanced variants of thermal proteome profiling etc. Why do you think it is like this? If these techniques are so great, why aren't they being used for actual science on a much greater scale? Or is my assumption wrong? Excited to listen to your views. For perspective, I am a cancer biologist trying to […]
  • 👋 Welcome to r/Peptidescamcompanies – Introduce Yourself and Read First!
    by /u/Icy_Race8562
    submitted by /u/Icy_Race8562 [link] [comments]
  • Regarding Journal of Proteome Research
    by /u/bluemooninvestor
    I have submitted a paper to JPR for the first time. It has been three weeks and the status is still "Editorial Review". Does the manuscript status change to Peer Review or something like that when it's under actual review? Or does it mean it's still with the editor only? submitted by /u/bluemooninvestor [link] [comments]

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