What is the default parameter of bootstrap value in kallisto tool at the quantification stage???What should be a good bootstrap value for rna-seq data?
The information is right there..
kallisto quant
kallisto 0.44.0
Computes equivalence classes for reads and quantifies abundances
Usage: kallisto quant [arguments] FASTQ-files
Required arguments:
-i, --index=STRING Filename for the kallisto index to be used for
quantification
-o, --output-dir=STRING Directory to write output to
Optional arguments:
--bias Perform sequence based bias correction
-b, --bootstrap-samples=INT Number of bootstrap samples (default: 0)
--seed=INT Seed for the bootstrap sampling (default: 42)
--plaintext Output plaintext instead of HDF5
--fusion Search for fusions for Pizzly
--single Quantify single-end reads
--single-overhang Include reads where unobserved rest of fragment is
predicted to lie outside a transcript
--fr-stranded Strand specific reads, first read forward
--rf-stranded Strand specific reads, first read reverse
-l, --fragment-length=DOUBLE Estimated average fragment length
-s, --sd=DOUBLE Estimated standard deviation of fragment length
(default: -l, -s values are estimated from paired
end data, but are required when using --single)
-t, --threads=INT Number of threads to use (default: 1)
--pseudobam Save pseudoalignments to transcriptome to BAM file
--genomebam Project pseudoalignments to genome sorted BAM file
-g, --gtf GTF file for transcriptome information
(required for --genomebam)
-c, --chromosomes Tab separated file with chrosome names and lengths
(optional for --genomebam, but recommended)
There is no correct or incorrect value to use. When I use Kallisto, I default to 50 bootstraps.
Note that the bootstrapped values are then output to the abundance.h5 file.
Kevin
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version 2.3.6
Thanks for the information