Project description:A natural way to benchmark the performance of an analytical experimental setup is to use samples of known content, and see to what degree one can correctly infer the content of such a sample from the data. For shotgun proteomics, one of the inherent problems of interpreting data is that the measured analytes are peptides and not the actual proteins themselves. As some proteins share proteolytic peptides, there might be more than one possible causative set of proteins resulting in a given set of peptides. Hence, there is a need for mechanisms that infer proteins from a list of detected peptides. Today's commercially available samples of known content do not expose these complications in protein inference, as their contained proteins deliberately are selected for producing tryptic peptides that are unique to a single protein. For a realistic benchmark of protein inference procedures, there is, therefore, a need for samples of known content where the present proteins share peptides with known absent proteins. Here, we present such a standard, based on E. coli expressed protein fragments.

Project description:Gene regulatory network inference is essential to uncover complex relationships among gene pathways and inform downstream experiments, ultimately enabling regulatory network re-engineering. Network inference from transcriptional time-series data requires accurate, interpretable, and efficient determination of causal relationships among thousands of genes. Here, we develop Bootstrap Elastic net regression from Time Series (BETS), a statistical framework based on Granger causality for the recovery of a directed gene network from transcriptional time-series data. BETS uses elastic net regression and stability selection from bootstrapped samples to infer causal relationships among genes. BETS is highly parallelized, enabling efficient analysis of large transcriptional data sets. We show competitive accuracy on a community benchmark, the DREAM4 100-gene network inference challenge, where BETS is one of the fastest among methods of similar performance and additionally infers whether the causal effects are activating or inhibitory. We apply BETS to transcriptional time-series data of 2,768 differentially-expressed genes from A549 cells exposed to glucocorticoids over a period of 12 hours. We identify a network of 2,768 genes and 31,945 directed edges (FDR <= 0.2). We validate inferred causal network edges using two external data sources: overexpression experiments on the same glucocorticoid system, and genetic variants associated with inferred edges in primary lung tissue in the Genotype-Tissue Expression (GTEx) v6 project. BETS is available as an open source software package at https://github.com/lujonathanh/BETS

Project description:Gene regulatory network inference is essential to uncover complex relationships among gene pathways and inform downstream experiments, ultimately enabling regulatory network re-engineering. Network inference from transcriptional time-series data requires accurate, interpretable, and efficient determination of causal relationships among thousands of genes. Here, we develop Bootstrap Elastic net regression from Time Series (BETS), a statistical framework based on Granger causality for the recovery of a directed gene network from transcriptional time-series data. BETS uses elastic net regression and stability selection from bootstrapped samples to infer causal relationships among genes. BETS is highly parallelized, enabling efficient analysis of large transcriptional data sets. We show competitive accuracy on a community benchmark, the DREAM4 100-gene network inference challenge, where BETS is one of the fastest among methods of similar performance and additionally infers whether the causal effects are activating or inhibitory. We apply BETS to transcriptional time-series data of 2,768 differentially-expressed genes from A549 cells exposed to glucocorticoids over a period of 12 hours. We identify a network of 2,768 genes and 31,945 directed edges (FDR <= 0.2). We validate inferred causal network edges using two external data sources: overexpression experiments on the same glucocorticoid system, and genetic variants associated with inferred edges in primary lung tissue in the Genotype-Tissue Expression (GTEx) v6 project. BETS is available as an open source software package at https://github.com/lujonathanh/BETS

Project description:This dataset is no actual new study but the results of the benchmark of the iPRG2008 benchmark dataset used in the manuscript "In-depth Analysis of Protein Inference Algorithms using a Workflow Framework and Well-Defined Metrics".

Project description:This dataset is no actual new study but the results of the benchmark of the iPRG2008 benchmark dataset used in the manuscript "In-depth Analysis of Protein Inference Algorithms using a Workflow Framework and Well-Defined Metrics".

Project description:This dataset is no actual new study but the results of the benchmark of the iPRG2008 benchmark dataset used in the manuscript "In-depth Analysis of Protein Inference Algorithms using a Workflow Framework and Well-Defined Metrics".

Project description:This dataset is no actual new study but the results of the benchmark of the iPRG2008 benchmark dataset used in the manuscript "In-depth Analysis of Protein Inference Algorithms using a Workflow Framework and Well-Defined Metrics".

Project description:Motivation: In bottom-up mass spectrometry proteins are enzymatically digested before measurement. The relationship between proteins and peptides can be represented by bipartite graphs that can be split into connected components. This representation is useful to aid protein inference and quantification, which is complex due to the occurrence of shared peptides. We conducted a comprehensive analysis of these bipartite graphs using peptides from an in silico digestion of protein databases as well as quantified peptides. Results: The graphs based on quantified peptides are smaller and have less complex structures compared to the database level. However, the proportion of protein nodes without unique peptides and the proportion of graphs that contain these proteins increase. Large differences between the different underlying organisms on database as well as quantitative level could be observed. Insights of this analysis may be useful for the development of protein inference and quantification algorithms. Link to preprint: https://www.biorxiv.org/content/10.1101/2021.07.28.454128v1?ct=

Project description:Motivation: In bottom-up mass spectrometry proteins are enzymatically digested before measurement. The relationship between proteins and peptides can be represented by bipartite graphs that can be split into connected components. This representation is useful to aid protein inference and quantification, which is complex due to the occurrence of shared peptides. We conducted a comprehensive analysis of these bipartite graphs using peptides from an in silico digestion of protein databases as well as quantified peptides. Results: The graphs based on quantified peptides are smaller and have less complex structures compared to the database level. However, the proportion of protein nodes without unique peptides and the proportion of graphs that contain these proteins increase. Large differences between the two underlying organisms (mouse and yeast) on database as well as quantitative level could be observed. Insights of this analysis may be useful for the development of protein inference and quantification algorithms. Link to preprint: https://www.biorxiv.org/content/10.1101/2021.07.28.454128v1?ct=

Project description:Motivation: In bottom-up mass spectrometry proteins are enzymatically digested before measurement. The relationship between proteins and peptides can be represented by bipartite graphs that can be split into connected components. This representation is useful to aid protein inference and quantification, which is complex due to the occurrence of shared peptides. We conducted a comprehensive analysis of these bipartite graphs using peptides from an in silico digestion of protein databases as well as quantified peptides. Results: The graphs based on quantified peptides are smaller and have less complex structures compared to the database level. However, the proportion of protein nodes without unique peptides and the proportion of graphs that contain these proteins increase. Large differences between the two underlying organisms (mouse and yeast) on database as well as quantitative level could be observed. Insights of this analysis may be useful for the development of protein inference and quantification algorithms. Link to preprint: https://www.biorxiv.org/content/10.1101/2021.07.28.454128v1?ct=