How many reads do I need? What's my sequencing depth? These are common questions I get all the time. Calculating how much sequence data you need to hit a target depth of coverage, or the inverse, what's the coverage depth given a set amount of sequencing, are both easy to answer with some basic algebra. Given one or the other, plus the genome size and read length/configuration, you can calculate either.
This is a guest post from VP Nagraj, a data scientist embedded within UVA’s Health Sciences Library, who runs our Data Analysis Support Hub (DASH) service. The What GRUPO (Gauging Research University Publication Output) is a Shiny app that provides side-by-side benchmarking of American research university publication activity.
Per tradition, Russ Altman gave his "Translational Bioinformatics: The Year in Review" presentation at the close of the AMIA Joint Summit on Translational Bioinformatics in San Francisco on March 26th. This year, papers came from six key areas (and a final Odds and Ends category). His full slide deck is available here.
I recently found this little gem of a web app that analyzes the clarity of your writing. Hemingway highlights long, complex, and hard to read sentences. It also highlights complex words where a simple one would do, and highlights adverbs, suggesting you use a stronger verb instead. It highlights passive voice (bad!), and tells you the minimum reading grade level necessary to understand your writing.
I collaborate with several investigators on gene expression projects using both microarray and RNA-seq. After I show a collaborator which genes are dysregulated in a particular condition or tissue, the most common question I get is " what are the transcription factors regulating these genes? " This isn't the easiest question to answer.
Many of you may be familiar with WebGestalt, a wonderful web utility developed by Bing Zhang at Vanderbilt for doing basic gene-set enrichment analyses. Last year, we invited Bing to speak at our annual retreat for the Vanderbilt Graduate Program in Human Genetics, and he did not disappoint! Bing walked us through his new tool called NetGestalt.
Two of the most common questions at the beginning of an RNA-seq experiments are "how many reads do I need?" and "how many replicates do I need?". This paper describes a web application for designing RNA-seq applications that calculates an appropriate sample size and read depth to satisfy user-defined criteria such as cost, maximum number of reads or replicates attainable, etc.
It's happened to all of us. You read about a new tool, database, webservice, software, or some interesting and useful data, but when you browse to http://instititution.edu/~home/professorX/lab/data, there's no trace of what you were looking for. THE PROBLEM This isn't an uncommon problem. See the following two articles: The first gives us some alarming statistics.
Recently published in Nucleic Acids Research: F. Zambelli, G. M. Prazzoli, G. Pesole, G. Pavesi, Cscan: finding common regulators of a set of genes by using a collection of genome-wide ChIP-seq datasets., Nucleic acids research 40 , W510–5 (2012). Cscan web interface screenshot This paper presents a methodology and software implementation that allows users to discover a set of transcription factors or epigenetic modifications that
Thanks to the excellent work of Lucia Hindorff and colleagues at NHGRI, the GWAS catalog provides a great reference for the cumulative results of GWAS for various phenotypes. Anyone familiar with GWAS also likely knows about dbGaP – the NCBI repository for genotype-phenotype relationships – and the wealth of data it contains.