Search icon CANCEL
Arrow left icon
Explore Products
Best Sellers
New Releases
Books
Videos
Audiobooks
Learning Hub
Conferences
Free Learning
Arrow right icon
Arrow up icon
GO TO TOP
R Bioinformatics Cookbook

You're reading from   R Bioinformatics Cookbook Use R and Bioconductor to perform RNAseq, genomics, data visualization, and bioinformatic analysis

Arrow left icon
Product type Paperback
Published in Oct 2019
Publisher Packt
ISBN-13 9781789950694
Length 316 pages
Edition 1st Edition
Languages
Tools
Arrow right icon
Authors (2):
Arrow left icon
Dr Dan Maclean Dr Dan Maclean
Author Profile Icon Dr Dan Maclean
Dr Dan Maclean
Dan MacLean Dan MacLean
Author Profile Icon Dan MacLean
Dan MacLean
Arrow right icon
View More author details
Toc

Table of Contents (13) Chapters Close

Preface 1. Performing Quantitative RNAseq 2. Finding Genetic Variants with HTS Data FREE CHAPTER 3. Searching Genes and Proteins for Domains and Motifs 4. Phylogenetic Analysis and Visualization 5. Metagenomics 6. Proteomics from Spectrum to Annotation 7. Producing Publication and Web-Ready Visualizations 8. Working with Databases and Remote Data Sources 9. Useful Statistical and Machine Learning Methods 10. Programming with Tidyverse and Bioconductor 11. Building Objects and Packages for Code Reuse 12. Other Books You May Enjoy

Performing Quantitative RNAseq

The technology of RNAseq has revolutionized the study of transcript abundances, bringing high-sensitivity detection and high-throughput analysis. Bioinformatic analysis pipelines using RNAseq data typically start with a read quality control step followed by either alignment to a reference or the assembly of sequence reads into longer transcripts de novo. After that, transcript abundances are estimated with read counting and statistical models and differential expression between samples is assessed. Naturally, there are many technologies available for all steps of this pipeline. The quality control and read alignment steps will usually take place outside of R, so analysis in R will begin with a file of transcript or gene annotations (such as GFF and BED files) and a file of aligned reads (such as BAM files).

The tools in R for performing analysis are powerful and flexible. Many of them are part of the Bioconductor suite and, as such, integrate together very nicely. The key question researchers wish to answer with RNAseq is usually: Which transcripts are differentially expressed? In this chapter, we'll look at some recipes for that in standard cases where we already know the genomic positions of genes we're interested in, and in cases where we need to find unannotated transcripts. We'll also look at other important recipes that help answer the questions How many replicates are enough? and Which allele is expressed more?

In this chapter, we will cover the following recipes:

  • Estimating differential expression with edgeR
  • Estimating differential expression with DESeq2
  • Power analysis with powsimR
  • Finding unannotated transcribed regions with GRanges objects
  • Finding regions showing high expression ab initio with bumphunter
  • Differential peak analysis
  • Estimating batch effects using SVA
  • Finding allele-specific expression with AllelicImbalance
  • Plotting and presenting RNAseq data
lock icon The rest of the chapter is locked
Register for a free Packt account to unlock a world of extra content!
A free Packt account unlocks extra newsletters, articles, discounted offers, and much more. Start advancing your knowledge today.
Unlock this book and the full library FREE for 7 days
Get unlimited access to 7000+ expert-authored eBooks and videos courses covering every tech area you can think of
Renews at £16.99/month. Cancel anytime