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OLIGONUCLEOTIDE LIGATION, BARCODING AND METHODS AND COMPOSITIONS FOR IMPROVING DATA QUALITY AND THROUGHPUT USING MASSIVELY PARALLEL SEQUENCING

机译：大规模并行测序技术改善寡核苷酸的结扎，编码，方法和组合物

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摘要

Described herein is a buffer concentration for highly efficient ligation of two oligonucleotides. The embodiments herein have led to the development of an optimized ligation step used in the sample preparation for sequencing reactions. Further, embodiments herein describe a high-throughput method for sequencing using barcodes or the purpose of multiplexing several samples simultaneously and novel methods for making targeted DNA libraries for re-sequencing on massively parallel next-generation sequencing platforms and for alternatives to gel-purification for recovering the desired templates from small RNA libraries for next generation sequencing.

机译：本文描述了用于两个寡核苷酸的高效连接的缓冲液浓度。本文的实施方案已导致开发用于测序反应的样品制备中的优化的连接步骤。此外，本文的实施方案描述了用于使用条形码测序或同时多路复用多个样品的目的的高通量方法，以及用于制备靶向DNA文库以在大规模平行的下一代测序平台上进行重测序以及用于凝胶纯化的替代方法的新颖方法。从小型RNA库中回收所需模板，以进行下一代测序。

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公开/公告号WO2011140510A3

专利类型
公开/公告日2012-03-29

原文格式PDF
申请/专利权人 BIOO SCIENTIFIC CORPORATION;TOLOUE MASOUD M.;GOLDRICK MARIANNA;
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申请/专利号WO2011US35633
发明设计人 TOLOUE MASOUD M.;GOLDRICK MARIANNA;
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申请日2011-05-06
分类号C12Q1/68;C12N15/10;C12N15/11;
国家 WO
入库时间 2022-08-21 17:18:59

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