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Proteomics Focused Bioinformatics Workshop 2021 - MaxQuant output and Limma results

  Рет қаралды 7,328

IDeA National Resource for Quantitative Proteomics

IDeA National Resource for Quantitative Proteomics

Күн бұрын

Пікірлер: 3
@svar-x3h
@svar-x3h 9 күн бұрын
As part of downstream analysis e.g. reactome, I need to use the protein IDs or gene names from my raw data. These downstream analysis dont work when there are multiple IDs per row hence they need to be separated with each protein having its own value. Since there are multiple IDs per row, do you assume that the Reporter intensity corrected value for each protein or gene in a given row is the same?
@noorfatima-gj8cb
@noorfatima-gj8cb 10 ай бұрын
Hi, from where we take the data which we use as a input?
@ideanationalresourceforqua4640
@ideanationalresourceforqua4640 10 ай бұрын
The input is from MaxQuant. Have you used MaxQuant before?
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