standardise: Standardisation
In PengyiYang/PhosR: A set of methods and tools for comprehensive analysis of phosphoproteomics data
Description
Usage
Arguments
Value
Examples
Description
Standardisation by z-score transformation.
Usage
1
standardise(mat)
Arguments
mat
a matrix with rows correspond to phosphosites and columns
correspond to samples.
Value
A standardised matrix
Examples
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data('phospho_L6_ratio')
data('SPSs')
grps = gsub('_.+', '', colnames(phospho.L6.ratio))
# Cleaning phosphosite label
phospho.site.names = rownames(phospho.L6.ratio)
L6.sites = gsub(' ', '', sapply(strsplit(rownames(phospho.L6.ratio), '~'),
function(x){paste(toupper(x[2]), x[3], '',
sep=';')}))
phospho.L6.ratio = t(sapply(split(data.frame(phospho.L6.ratio), L6.sites),
colMeans))
phospho.site.names = split(phospho.site.names, L6.sites)
# Construct a design matrix by condition
design = model.matrix(~ grps - 1)
# phosphoproteomics data normalisation using RUV
ctl = which(rownames(phospho.L6.ratio) %in% SPSs)
phospho.L6.ratio.RUV = RUVphospho(phospho.L6.ratio, M = design, k = 3,
ctl = ctl)
phosphoL6 = phospho.L6.ratio.RUV
rownames(phosphoL6) = phospho.site.names
# filter for up-regulated phosphosites
phosphoL6.mean <- meanAbundance(phosphoL6, grps = gsub('_.+', '',
colnames(phosphoL6)))
aov <- matANOVA(mat=phosphoL6, grps=gsub('_.+', '', colnames(phosphoL6)))
phosphoL6.reg <- phosphoL6[(aov < 0.05) &
(rowSums(phosphoL6.mean > 0.5) > 0),,drop = FALSE]
L6.phos.std <- standardise(phosphoL6.reg)
PengyiYang/PhosR documentation built on June 21, 2020, 8:37 a.m.
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Description Usage Arguments Value Examples
Description
Standardisation by z-score transformation.
Usage
1 | standardise(mat)
|
Arguments
mat |
a matrix with rows correspond to phosphosites and columns correspond to samples. |
Value
A standardised matrix
Examples
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 29 30 31 | data('phospho_L6_ratio')
data('SPSs')
grps = gsub('_.+', '', colnames(phospho.L6.ratio))
# Cleaning phosphosite label
phospho.site.names = rownames(phospho.L6.ratio)
L6.sites = gsub(' ', '', sapply(strsplit(rownames(phospho.L6.ratio), '~'),
function(x){paste(toupper(x[2]), x[3], '',
sep=';')}))
phospho.L6.ratio = t(sapply(split(data.frame(phospho.L6.ratio), L6.sites),
colMeans))
phospho.site.names = split(phospho.site.names, L6.sites)
# Construct a design matrix by condition
design = model.matrix(~ grps - 1)
# phosphoproteomics data normalisation using RUV
ctl = which(rownames(phospho.L6.ratio) %in% SPSs)
phospho.L6.ratio.RUV = RUVphospho(phospho.L6.ratio, M = design, k = 3,
ctl = ctl)
phosphoL6 = phospho.L6.ratio.RUV
rownames(phosphoL6) = phospho.site.names
# filter for up-regulated phosphosites
phosphoL6.mean <- meanAbundance(phosphoL6, grps = gsub('_.+', '',
colnames(phosphoL6)))
aov <- matANOVA(mat=phosphoL6, grps=gsub('_.+', '', colnames(phosphoL6)))
phosphoL6.reg <- phosphoL6[(aov < 0.05) &
(rowSums(phosphoL6.mean > 0.5) > 0),,drop = FALSE]
L6.phos.std <- standardise(phosphoL6.reg)
|
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