RAPID WHOLE GENOME AMPLIFICATION
    1.
    发明申请
    RAPID WHOLE GENOME AMPLIFICATION 有权
    快速全基因扩增

    公开(公告)号:US20120171726A1

    公开(公告)日:2012-07-05

    申请号:US13339633

    申请日:2011-12-29

    IPC分类号: C12P19/34 C12N9/12

    摘要: The present invention provides compositions and methods for rapidly amplifying target nucleic acid (e.g., using whole genome amplification) that allows small amounts of starting nucleic acid to be employed. In certain embodiments, the methods employ compositions that comprise: phi29 polymerase, exo- Klenow polymerase and/or Klenow polymerase, dNTPs, primers, and a buffering agent. In some embodiments, the target nucleic acid is amplified at a rate that would result in at least 1000-fold amplification in thirty minutes.

    摘要翻译: 本发明提供用于快速扩增允许使用少量起始核酸的靶核酸(例如,使用全基因组扩增)的组合物和方法。 在某些实施方案中,所述方法使用包含以下的组合物:phi29聚合酶,ex-Klenow聚合酶和/或Klenow聚合酶,dNTP,引物和缓冲剂。 在一些实施方案中,以在30分钟内至少产生1000倍扩增的速率扩增靶核酸。

    Rapid whole genome amplification
    3.
    发明授权
    Rapid whole genome amplification 有权
    快速全基因组扩增

    公开(公告)号:US09428801B2

    公开(公告)日:2016-08-30

    申请号:US13339633

    申请日:2011-12-29

    IPC分类号: C12P19/34 C12Q1/68

    摘要: The present invention provides compositions and methods for rapidly amplifying target nucleic acid (e.g., using whole genome amplification) that allows small amounts of starting nucleic acid to be employed. In certain embodiments, the methods employ compositions that comprise: phi29 polymerase, exo- Klenow polymerase and/or Klenow polymerase, dNTPs, primers, and a buffering agent. In some embodiments, the target nucleic acid is amplified at a rate that would result in at least 1000-fold amplification in thirty minutes.

    摘要翻译: 本发明提供用于快速扩增允许使用少量起始核酸的靶核酸(例如,使用全基因组扩增)的组合物和方法。 在某些实施方案中,所述方法使用包含以下的组合物:phi29聚合酶,ex-Klenow聚合酶和/或Klenow聚合酶,dNTP,引物和缓冲剂。 在一些实施方案中,以在30分钟内至少产生1000倍扩增的速率扩增靶核酸。

    Multiple displacement amplification

    公开(公告)号:US09890408B2

    公开(公告)日:2018-02-13

    申请号:US12905819

    申请日:2010-10-15

    IPC分类号: C12Q1/64 C12P19/34 C12Q1/68

    摘要: The present invention provides methods kits and systems for performing multiple displacement amplification reactions. In one method a sample of nucleic acid is provided. The nucleic acid is contacted with a reaction mixture which includes a set of oligonucleotide primers, a one or more polymerase enzymes and a detergent. The reaction mixture is then subjected to conditions under which the nucleic acid sequence is amplified to produce an amplified product in a multiple displacement reaction. The method may also be carried out by contacting the nucleic acid with the reaction mixture in the form of an emulsion. A kit is also provided for carrying out either the methods described above. The kit includes one or more polymerases, a plurality of primers and a detergent. The kit may also include a hydrophobic polymer and may include instructions for performing a multiple displacement amplification reaction on a nucleic acid sample.