readPanels: Import GenMapper Panels configuration file
In seqinr: Biological Sequences Retrieval and Analysis
readPanels R Documentation
Import GenMapper Panels configuration file
Description
In a Panel configuration file there is a description for a given identification
kit of the marker names, their dye label color, expected size range,
expected positive control genotypes, number of bases in core repeat,
stutter percentages, and allele names.
Usage
readPanels(file,
colnames = c("marker", "dye.col", "min.bp", "max.bp", "exp.pcg", "repeat.bp",
"stutter.pc", "uknw", "allele names"))
Arguments
file
The name of the Panel configuration file.
colnames
The names to be used for the columns of the data.frames.
Details
Number of bases in core repeat is set to 9 for Amelogenin locus.
Value
A list whose first element is the file header info and following elements
data.frames, one for each kit encountered in the file.
Author(s)
J.R. Lobry
References
citation("seqinR")
See Also
readBins, plotPanels.
Examples
#
# Check that we can read the 2 exemple files in the seqinR package:
#
path1 <- system.file("abif/AmpFLSTR_Panels_v1.txt", package = "seqinr")
res1 <- readPanels(path1)
path2 <- system.file("abif/Promega_Panels_v1.txt", package = "seqinr")
res2 <- readPanels(path2)
#
# Show the kits described in res1:
#
names(res1)
#
# Show some data for a given kit:
#
res1[["Identifiler_v1"]][, 1:7]
#
# Plot a simple summary of two kits:
#
par(mfrow = c(2,1))
plotPanels("Identifiler_v1", res1)
plotPanels("PowerPlex_16_v1", res2)
#
# Simple quality check since seqinR 2.0-4 with a file which containing
# a non constant number of tabulations as separator:
#
path3 <- system.file("abif/Prototype_PowerPlex_EP01_Pa.txt", package = "seqinr")
res3 <- readPanels(path3)
seqinr documentation built on March 31, 2023, 3:05 p.m.
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| readPanels | R Documentation |
Import GenMapper Panels configuration file
Description
In a Panel configuration file there is a description for a given identification kit of the marker names, their dye label color, expected size range, expected positive control genotypes, number of bases in core repeat, stutter percentages, and allele names.
Usage
readPanels(file,
colnames = c("marker", "dye.col", "min.bp", "max.bp", "exp.pcg", "repeat.bp",
"stutter.pc", "uknw", "allele names"))Arguments
file |
The name of the Panel configuration file. |
colnames |
The names to be used for the columns of the data.frames. |
Details
Number of bases in core repeat is set to 9 for Amelogenin locus.
Value
A list whose first element is the file header info and following elements data.frames, one for each kit encountered in the file.
Author(s)
J.R. Lobry
References
citation("seqinR")
See Also
readBins, plotPanels.
Examples
#
# Check that we can read the 2 exemple files in the seqinR package:
#
path1 <- system.file("abif/AmpFLSTR_Panels_v1.txt", package = "seqinr")
res1 <- readPanels(path1)
path2 <- system.file("abif/Promega_Panels_v1.txt", package = "seqinr")
res2 <- readPanels(path2)
#
# Show the kits described in res1:
#
names(res1)
#
# Show some data for a given kit:
#
res1[["Identifiler_v1"]][, 1:7]
#
# Plot a simple summary of two kits:
#
par(mfrow = c(2,1))
plotPanels("Identifiler_v1", res1)
plotPanels("PowerPlex_16_v1", res2)
#
# Simple quality check since seqinR 2.0-4 with a file which containing
# a non constant number of tabulations as separator:
#
path3 <- system.file("abif/Prototype_PowerPlex_EP01_Pa.txt", package = "seqinr")
res3 <- readPanels(path3)
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We want your feedback!
Note that we can't provide technical support on individual packages. You should contact the package authors for that.
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