The presence of duplicates introduced by PCR amplification is a major issue in paired short reads from next-generation sequencing platforms. These duplicates might have a serious impact on research applications, such as scaffolding in whole-genome sequencing and discovering large-scale genome variations, and are usually removed. We present FastUniq as a fast de novo tool for removal of duplicates in paired short reads. FastUniq identifies duplicates by comparing sequences between read pairs and does not require complete genome sequences as prerequisites. FastUniq is capable of simultaneously handling reads with different lengths and results in highly efficient running time, which increases linearly at an average speed of 87 million reads pe...
Background: RNA-seq and small RNA-seq are powerful, quantitative tools to study gene regulation and ...
International audienceLinked reads technologies, such as the 10X chromium system, use microfluidics ...
BACKGROUND: The first step of virtually all next generation sequencing analysis involves the splitti...
<div><p>The presence of duplicates introduced by PCR amplification is a major issue in paired short ...
The presence of duplicates introduced by PCR amplification is a major issue in paired short reads fr...
Background: The first step of virtually all next generation sequencing analysis involves the splitti...
Abstract Background Next generation sequencing datasets are stored as FASTQ formatted files. In orde...
The increasingly widespread use of next generation sequencing protocols has brought the need for the...
This is a pre-copyedited, author-produced version of an article accepted for publication in Bioinfor...
BackgroundRNA sequencing (RNA-seq) has become the standard means of analyzing gene and transcript ex...
<p>(A) The number of read pairs before and after duplicates removal using FastUniq or the mapping-ba...
DNA sequencing analysis typically involves mapping reads to just one reference genome. Mapping again...
Background: During library construction polymerase chain reaction is used to enrich the DNA before s...
Removing duplicate and near-duplicate reads, generated by high-throughput sequencing technologies, i...
Several methods for ultra-high throughput DNA sequencing are currently under investigation. Many of ...
Background: RNA-seq and small RNA-seq are powerful, quantitative tools to study gene regulation and ...
International audienceLinked reads technologies, such as the 10X chromium system, use microfluidics ...
BACKGROUND: The first step of virtually all next generation sequencing analysis involves the splitti...
<div><p>The presence of duplicates introduced by PCR amplification is a major issue in paired short ...
The presence of duplicates introduced by PCR amplification is a major issue in paired short reads fr...
Background: The first step of virtually all next generation sequencing analysis involves the splitti...
Abstract Background Next generation sequencing datasets are stored as FASTQ formatted files. In orde...
The increasingly widespread use of next generation sequencing protocols has brought the need for the...
This is a pre-copyedited, author-produced version of an article accepted for publication in Bioinfor...
BackgroundRNA sequencing (RNA-seq) has become the standard means of analyzing gene and transcript ex...
<p>(A) The number of read pairs before and after duplicates removal using FastUniq or the mapping-ba...
DNA sequencing analysis typically involves mapping reads to just one reference genome. Mapping again...
Background: During library construction polymerase chain reaction is used to enrich the DNA before s...
Removing duplicate and near-duplicate reads, generated by high-throughput sequencing technologies, i...
Several methods for ultra-high throughput DNA sequencing are currently under investigation. Many of ...
Background: RNA-seq and small RNA-seq are powerful, quantitative tools to study gene regulation and ...
International audienceLinked reads technologies, such as the 10X chromium system, use microfluidics ...
BACKGROUND: The first step of virtually all next generation sequencing analysis involves the splitti...