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Detection of microRNAs in color space

机译:检测色彩空间中的microRNA

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Motivation: Deep sequencing provides inexpensive opportunities to characterize the transcriptional diversity of known genomes. The AB SOLiD technology generates millions of short sequencing reads in color-space; that is, the raw data is a sequence of colors, where each color represents 2 nt and each nucleotide is represented by two consecutive colors. This strategy is purported to have several advantages, including increased ability to distinguish sequencing errors from polymorphisms. Several programs have been developed to map short reads to genomes in color space. However, a number of previously unexplored technical issues arise when using SOLiD technology to characterize microRNAs. Results: Here we explore these technical difficulties. First, since the sequenced reads are longer than the biological sequences, every read is expected to contain linker fragments. The color-calling error rate increases toward the 3(') end of the read such that recognizing the linker sequence for removal becomes problematic. Second, mapping in color space may lead to the loss of the first nucleotide of each read. We propose a sequential trimming and mapping approach to map small RNAs. Using our strategy, we reanalyze three published insect small RNA deep sequencing datasets and characterize 22 new microRNAs. Availability and implementation: A bash shell script to perform the sequential trimming and mapping procedure, called SeqTrimMap, is available at: www.mirbase.org/tools/seqtrimmap/
机译:动机:深度测序提供了廉价的机会来表征已知基因组的转录多样性。 AB SOLiD技术可在色彩空间中生成数百万个短序列读取;也就是说,原始数据是一系列颜色,其中每种颜色表示2 nt,每个核苷酸由两种连续的颜色表示。该策略据称具有几个优点,包括提高了区分序列错误和多态性的能力。已经开发了一些程序来将短读物映射到色彩空间中的基因组。但是,使用SOLiD技术表征microRNA时,会出现许多以前未曾探索的技术问题。结果:在这里我们探索这些技术难题。首先,由于测序的读段比生物学序列长,因此预期每个读段都包含接头片段。显色错误率朝向读取的3(')端增加,因此识别要除去的接头序列变得有问题。其次,在色彩空间中进行映射可能会导致每次读取的第一个核苷酸丢失。我们提出了一种顺序修剪和定位方法来定位小RNA。使用我们的策略,我们重新分析了三个已发布的昆虫小RNA深度测序数据集,并表征了22种新的microRNA。可用性和实现:www.mirbase.org/tools/seqtrimmap/提供了一个用于执行顺序修整和映射过程的bash shell脚本,称为SeqTrimMap。

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