发明公开
EP1216100A1 REACTION SYSTEM FOR PERFORMING IN THE AMPLIFICATION OF NUCLEIC ACIDS
审中-公开
反应体系的具体实施的核酸扩增
- 专利标题: REACTION SYSTEM FOR PERFORMING IN THE AMPLIFICATION OF NUCLEIC ACIDS
- 专利标题(中): 反应体系的具体实施的核酸扩增
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申请号: EP00964445.1申请日: 2000-09-29
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公开(公告)号: EP1216100A1公开(公告)日: 2002-06-26
- 发明人: LEE, Martin, Alan , BIRD, Hilary , LESLIE, Dario, LyallCBD Porton Down , SQUIRRELL, David, James , SHAW, JohnCentral Research Laboratories Limited , WENN, DavidCentral Research Laboratories Limited , DEACON,JulieCentral Research Laboratories Limited
- 申请人: The Secretary of State For Defence in Her Britannic Majesty's Government of The United Kingdom of Great Britain and N. Ireland
- 申请人地址: CBD Porton Down Salisbury,Wiltshire SP4 0JQ GB
- 专利权人: The Secretary of State For Defence in Her Britannic Majesty's Government of The United Kingdom of Great Britain and N. Ireland
- 当前专利权人: The Secretary of State For Defence in Her Britannic Majesty's Government of The United Kingdom of Great Britain and N. Ireland
- 当前专利权人地址: CBD Porton Down Salisbury,Wiltshire SP4 0JQ GB
- 代理机构: Skelton, Stephen Richard
- 优先权: GB9922971 19990929
- 国际公布: WO0123093 20010405
- 主分类号: B01L7/00
- IPC分类号: B01L7/00 ; B01L3/00 ; C12Q1/68
摘要:
A method of carrying out an amplification reaction, said method comprising supplying to a well in a disposable unit (a) a sample which contains or is suspected of containing a target nucleic acid sequence (b) primers, nucleotides and enzymes required to effect said amplification reaction and (c) a buffer system, and subjecting the unit to thermal cycling conditions such that any target nucleic acid present within the sample is amplified; wherein the disposable unit comprises a thermally conducting layer and a facing layer having one or more reagent wells of up to 1000 microns in depth defined therebetween; and the reaction mixture comprises at least one of the following: A) a buffer system wherein the pH is above 8.3; B) a detergent; and/or C) a blocking agent. Apparatus for effecting the method as well as disposable units for use in the method are described. The method is particularly suitable for rapid PCR reactions.
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