inst/script/run_trip_rscript.R
In iofeidis/tripr: T-cell Receptor/Immunoglobulin Profiler (TRIP)
#!/usr/bin/env Rscript
# For Rscript on Windows cmd
# $> Rscript run_trip_rscript.R
# # If it doesn't work, you have to find the path to Rscript
# $> path\to\Rscript.exe" path\to\run_trip_rscript.R
library(tripr)
message("See run_TRIP() documentation by typing '?tripr::run_TRIP'")
# Change the default values with your preferred ones
run_TRIP(
# Replace the datapath with yours like (if it's on your working directory):
# datapath=fs::path_wd("dataset"),
datapath=fs::path_package("extdata", "dataset", package="tripr"),
output_path=fs::path_home("Documents/tripr_output"),
filelist=c("1_Summary.txt", "2_IMGT-gapped-nt-sequences.txt",
"4_IMGT-gapped-AA-sequences.txt", "6_Junction.txt"),
cell="Bcell",
throughput="High Throughput",
preselection="1,4C:W",
selection="5",
identity_range="85:100",
vgenes="",
dgenes="",
jgenes="",
cdr3_length_range="",
aminoacid="",
pipeline="1",
select_clonotype="V Gene + CDR3 Amino Acids",
highly_sim_params=paste0("1-1 2-1 3-1 4-1 5-1 6-1 7-1 8-1 9-1 10-1 11-1 ",
"12-1 13-1 14-1 15-2 16-2 17-2 18-2 19-2 20-2 21-2 23-2 24-2 25-2 ",
"26-2 27-2 28-2 29-3 30-3 31-3 32-3 33-3 34-3 35-3 36-3 37-3 38-3 ",
"39-3 40-3 41-3 42-3 43-3 44-3 45-3 46-3 47-3 48-3 49-3 50-3,1,Yes"),
shared_clonotypes_params="reads,1,Yes",
highly_shared_clonotypes_params="reads,1,Yes",
repertoires_params="1,4,6",
identity_groups="85:97,97:99,99:100,100:100",
multiple_values_params="2:7,2:3,2:5,2:11",
alignment_params="1,both,1,2:20",
mutations_params="both,0.5,0.5,2:20")
iofeidis/tripr documentation built on Dec. 20, 2021, 7:58 p.m.
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#!/usr/bin/env Rscript
# For Rscript on Windows cmd
# $> Rscript run_trip_rscript.R
# # If it doesn't work, you have to find the path to Rscript
# $> path\to\Rscript.exe" path\to\run_trip_rscript.R
library(tripr)
message("See run_TRIP() documentation by typing '?tripr::run_TRIP'")
# Change the default values with your preferred ones
run_TRIP(
# Replace the datapath with yours like (if it's on your working directory):
# datapath=fs::path_wd("dataset"),
datapath=fs::path_package("extdata", "dataset", package="tripr"),
output_path=fs::path_home("Documents/tripr_output"),
filelist=c("1_Summary.txt", "2_IMGT-gapped-nt-sequences.txt",
"4_IMGT-gapped-AA-sequences.txt", "6_Junction.txt"),
cell="Bcell",
throughput="High Throughput",
preselection="1,4C:W",
selection="5",
identity_range="85:100",
vgenes="",
dgenes="",
jgenes="",
cdr3_length_range="",
aminoacid="",
pipeline="1",
select_clonotype="V Gene + CDR3 Amino Acids",
highly_sim_params=paste0("1-1 2-1 3-1 4-1 5-1 6-1 7-1 8-1 9-1 10-1 11-1 ",
"12-1 13-1 14-1 15-2 16-2 17-2 18-2 19-2 20-2 21-2 23-2 24-2 25-2 ",
"26-2 27-2 28-2 29-3 30-3 31-3 32-3 33-3 34-3 35-3 36-3 37-3 38-3 ",
"39-3 40-3 41-3 42-3 43-3 44-3 45-3 46-3 47-3 48-3 49-3 50-3,1,Yes"),
shared_clonotypes_params="reads,1,Yes",
highly_shared_clonotypes_params="reads,1,Yes",
repertoires_params="1,4,6",
identity_groups="85:97,97:99,99:100,100:100",
multiple_values_params="2:7,2:3,2:5,2:11",
alignment_params="1,both,1,2:20",
mutations_params="both,0.5,0.5,2:20")
R Package Documentation
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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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