Author: Nathalie Pamir; Calvin Pan; Deanna L. Plubell; Patrick M. Hutchins; Chongren Tang; Jake Wimberger; Angela Irwin; Thomas Q. de Aguiar Vallim; Jay W. Heinecke; Aldons J. Lusis
Title: Genetic control of the HDL proteome Document date: 2018_8_31
ID: hx7n4xfo_35
Snippet: . CC-BY-NC-ND 4.0 International license is made available under a The copyright holder for this preprint (which was not peer-reviewed) is the author/funder. Figure 3 . Hierarchical clustering of the HDL metrics: Proteome, sterol efflux, particle concentration and size. min.MF, plus.MF, delta.BHK are unstimulated, ABCA1 upregulated and ABCA1 specific sterol efflux from BHK cells respectively. min.cAMP, plus.cAMP, delta.J774 are unstimulated, ABCA1.....
Document: . CC-BY-NC-ND 4.0 International license is made available under a The copyright holder for this preprint (which was not peer-reviewed) is the author/funder. Figure 3 . Hierarchical clustering of the HDL metrics: Proteome, sterol efflux, particle concentration and size. min.MF, plus.MF, delta.BHK are unstimulated, ABCA1 upregulated and ABCA1 specific sterol efflux from BHK cells respectively. min.cAMP, plus.cAMP, delta.J774 are unstimulated, ABCA1 upregulated and ABCA1 specific sterol efflux from J774 cells respectively. m.hdl.size and l.hdl.size are medium and large HDL sizes respectively. The correlation structure was determined using pearson correlation. The protein functional groups were curated from DAVID, KEGG, Panther, and Uniprot databases. Figure 1 . Self-loops were removed and edges were bundled for clarity. Node locations are assigned using an edge-weighted spring-embedded layout algorithm using the negative log of the Benjamini-Hochberg corrected p-value, and edge transparency is directly proportional to the same value. Red: negative correlation, Blue: positive correlation. Shorter distances indicate stronger correlations. Figure 1 : The heatmap visualization of the HDL protein abundances (calculated as normalized to total PSMs) across 93 strains. The proteins, their biological functions and cellular locations are represented. Logarithmic transformation of the total PSM normalized data has been performed to accommodate the abundance distribution form high (red) to very low (dark blue). White squares represent not available values. Both the proteins and the strains were clustered using Euclidean distances.
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