KR20010033130A - 핵산 서열화를 위한 질량 분광분석 방법 - Google Patents
핵산 서열화를 위한 질량 분광분석 방법 Download PDFInfo
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- KR20010033130A KR20010033130A KR1020007006503A KR20007006503A KR20010033130A KR 20010033130 A KR20010033130 A KR 20010033130A KR 1020007006503 A KR1020007006503 A KR 1020007006503A KR 20007006503 A KR20007006503 A KR 20007006503A KR 20010033130 A KR20010033130 A KR 20010033130A
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Abstract
Description
| 6-머 RNA(%) | 닉으로 정지된 RNA(%) | 완전한 길이의 RNA(%) | 닉 우회 효율(%) | |
| 참조 | 320±93 | - | (100) | 100±0 |
| 1N+7U | 193.2±46.3 | 12.45.4 | 95.8±6.5 | 88.5±5.1 |
| 1N+8U | 187.4±39.9 | 5.3±4.2 | 87.1±4.3 | 94.3±0.5 |
| 1N+9U | 232.7±45.6 | 10.1±1.1 | 65.7±4.4 | 87.6±1.8 |
| 1N+19U | 279.6±33.8 | 6.6±0.3 | 64.8±4.5 | 90.9±0.4 |
Claims (44)
- a) 고체 지지체상에 고정되어 있는, 프로모터와 프로모터에 작동가능하게 연결되어 있는 표적 핵산 서열을 포함하는 핵산 분자를 제공하고;b) 프로모터를 인지하는 RNA 폴리머라제를 사용하여 표적으로부터 한벌의 RNA 전사체 셋트를 생성하는 조건하에 프로모터 함유 핵산 분자를 전사시키며;c) 질량 분광분석법에 의해 전사체의 분자량 값을 측정하여 표적 분자의 핵산 서열을 결정함을 포함하여, 표적 핵산 분자의 서열을 결정하는 방법.
- 제1항에 있어서, 프로모터 함유 핵산 분자가 암호화 쇄의 5' 말단 또는 비암호화 쇄의 3' 말단을 통해 고정되는 방법.
- 제1항에 있어서, 핵산이 DNA 또는 PNA인 방법.
- 제1항 내지 제3항 중의 어느 한 항에 있어서, 암호화 쇄 및 비암호화 쇄를 갖는 핵산 프로모터 함유 프로브를 표적 핵산 서열을 포함하는 핵산 분자와 하이브리드화시키고, 이때 하이브리드화가 프로모터 함유 프로브의 일본쇄 영역과 표적을 포함하는 분자의 한쪽 말단 부위의 상보적인 일본쇄 영역 사이에서 발생됨으로써, 프로모터 및 표적을 포함하는 핵산 분자가 제조되는 방법.
- 제4항에 있어서, 표적을 포함하는 분자가 일본쇄이고, 상보적 일본쇄 영역을 포함하는 부분이 표적 함유 분자의 3'-말단에 있으며, 프로모터 함유 프로브 분자가 암호화 쇄의 3' 말단에 표적 함유 분자의 일본쇄 부분에 상보적인 5개 이상의 연속적인 뉴클레오타이드의 일본쇄 영역을 갖는 이본쇄인 방법.
- 제4항에 있어서, 표적을 포함하는 분자가, 프로모터 함유 분자의 일본쇄 부분에 상보적인 5개 이상의 연속적인 뉴클레오타이드를 포함하는 일본쇄 영역이 한쪽 말단에 있는 것을 제외하고는 이본쇄이고, 프로모터 함유 분자의 일본쇄 부분이 프로모터에 대해 동일한 말단에 있어 표적 함유 분자상에 일본쇄 영역이 존재하는 방법.
- 제4항 내지 제6항 중의 어느 한 항에 있어서, 표적 함유 분자와 하이브리드화하기 전에, 프로모터 함유 분자를 고체 지지체상에 고정시키는 방법.
- 제4항 내지 제6항 중의 어느 한 항에 있어서, 프로모터 함유 분자를 고체 지지체상에 고정시키기 전에 하이브리드화를 수행하는 방법.
- 제4항 내지 제8항 중의 어느 한 항에 있어서, 생성된 분자중의 닉을 RNA 폴리머라제로 전사시키기 전에 연결시키는 방법.
- 제1항 내지 제9항 중의 어느 한 항에 있어서, 프로모터 및 표적 핵산을 포함하는 핵산 분자를 RNA 폴리머라제로 전사시켜 염기 특이적으로 종결된 다수의 RNA 전사체를 생성하는 방법.
- 제1항 내지 제9항 중의 어느 한 항에 있어서, 프로모터 및 표적 핵산을 포함하는 핵산 분자를 RNA 폴리머라제로 전사시켜 RNA 전사체 셋트를 생성한 다음, 염기 특이적 리보뉴클레아제로 특이적으로 분해시켜 분해된 단편 셋트를 생성하고, 이의 분자량을 질량 분광분석법으로 평가하는 방법.
- 제1항 내지 제11항 중의 어느 한 항에 있어서, 표적 핵산 모두 또는 일부의 서열이 RNA 전사체에 의해 분자량에 따라 결정되는 방법.
- 제1항 내지 제12항 중의 어느 한 항에 있어서, 프로모터 또는 프로모터의 상보체를 포함하는 일본쇄 분자를 고정시키고, 이의 상보체를 포함하는 단편을 하이브리드화하여, 프로모터 및 5개 이상의 뉴클레오타이드 일본쇄 부분을 함유하는 이본쇄 영역을 포함하는 분자를 생성함으로써, 프로모터를 포함하는 핵산 분자를 제조하는 방법.
- 제1항 내지 제13항 중의 어느 한 항에 있어서, 프로모터가 파지, 진핵세포 및 원핵세포 프로모터로 이루어진 그룹으로부터 선택되는 방법.
- 제14항에 있어서, 프로모터가 아키박테리아, 유박테리아, 박테리오파지, DNA 바이러스, RNA 바이러스, 식물, 식물 바이러스 및 동물 프로모터로부터 선택되는 방법.
- 제1항 내지 제15항 중의 어느 한 항에 있어서, RNA 폴리머라제가 DNA 의존적 RNA 폴리머라제 또는 RNA 의존적 RNA 폴리머라제인 방법.
- 제1항 내지 제16항 중의 어느 한 항에 있어서, RNA 폴리머라제가 파지, 진핵세포 및 원핵세포 폴리머라제로 이루어진 그룹으로부터 선택되는 방법.
- 제17항에 있어서, 폴리머라제가 아키박테리아, 유박테리아, 박테리오파지, DNA 바이러스, RNA 바이러스, 식물, 식물 바이러스 및 동물 폴리머라제로부터 선택되는 방법.
- 제1항 내지 제18항 중의 어느 한 항에 있어서, RNA 폴리머라제가 에스케리키아 콜라이(Escherichia coli) RNA 폴리머라제, T7 RNA 폴리머라제, SP6 RNA 폴리머라제, T3 RNA 폴리머라제 및 Qβ 리플리카제로 이루어진 그룹으로부터 선택되는 방법.
- 제1항 내지 제19항 중의 어느 한 항에 있어서, 핵산을 고정시키기 전에, 지지체 표면을 아미노실란과 반응시켜 지지체를 유도체화시킴으로써 지지체의 표면에 1급 아민을 생성시키는 방법.
- 제20항에 있어서, 아미노실란이 3-아미노프로필트리에톡시실란인 방법.
- 제21항에 있어서, 지지체의 표면상의 1급 아민을 티올 반응성 가교결합제와 반응시켜 티올 반응성 고체 지지체를 형성함을 추가로 포함하는 방법.
- 제22항에 있어서, 티올 반응성 가교결합제가 N-석신이미딜 (4-요오도아세틸) 아미노벤조에이트(SIAB)인 방법.
- 제22항에 있어서, 유리 5'- 또는 3'-티올 그룹을 갖는 핵산 프로브와 티올 반응성 고체 지지체를 반응시켜 티올 그룹과 티올 반응성 고체 지지체 사이에 공유 결합을 형성시킴으로써 핵산 프로브를 고체 지지체에 고정시키는 방법.
- 제1항 내지 제21항 중의 어느 한 항에 있어서, 핵산 분자를 공유 연결에 의해 20fmol/㎟ 이상의 밀도로 고체 지지체의 표면에 고정시키는 방법.
- 제1항 내지 제25항 중의 어느 한 항에 있어서, 핵산이 정렬 형태로 고체 지지체의 표면상에 고정되는 방법.
- 제1항 내지 제26항 중의 어느 한 항에 있어서, 고체 지지체가 실리콘 또는 실리콘 피복되는 방법.
- 제1항 내지 제27항 중의 어느 한 항에 있어서, 표면이 고정된 핵산 분자를 함유하는 다수의 웰을 포함하는 방법.
- 제28항에 있어서, 웰이 조악한 내부 표면을 갖는 방법.
- 제28항에 있어서, 고체 지지체가 조악한 표면을 갖는 방법.
- 제28항에 있어서, 웰의 표면이 함몰된(pitted) 방법.
- 제1항 내지 제31항 중의 어느 한 항에 있어서, 전사 반응이 리보뉴클레오사이드 트리포스페이트 유사체의 존재하에 수행되어 리보뉴클레오사이드 트리포스파타제로부터 형성되는 RNA 전사체에 비해 생성된 RNA 전사체의 2차 구조가 감소되거나 RNA 폴리머라제 효소의 종결 및 턴오버의 엄수가 증가되는 방법.
- 제32항에 있어서, 전사 반응이 이노신 5'-트리포스페이트(ITP), 4-티오 우리딘 5'트리포스페이트(UTP), 5-브로모 UTP 및 5'-요오도 CTP로부터 선택되는 하나 이상의 유사체를 포함하는 방법.
- 제1항 내지 제33항 중의 어느 한 항에 있어서, 핵산이 링커를 통해 고체 지지체에 고정되는 방법.
- 제34항에 있어서, 링커에 의해 형성되는 연결이 가역적인 방법.
- 제34항에 있어서, 링커에 의해 형성되는 연결이 비가역적인 방법.
- 제34항에 있어서, 링커에 의해 형성되는 연결이 광 불안정성, 산 불안정성 또는 화학적으로 분해가능한 방법.
- 제1항 내제 제37항 중의 어느 한 항에 있어서, 하나 이상의 3'-데옥시리보뉴클레오타이드의 존재하에 전사가 수행되는 방법.
- 제1항 내지 제38항 중의 어느 한 항에 있어서, 핵산을 고정시키기 전 또는 후에, 질량분광분석용 매트릭스 물질을 지지체의 표면에 가하는 것을 추가로 포함하는 방법.
- 제1항 내지 제39항 중의 어느 한 항에 있어서, 질량 분광분석을 수행하기 전에 RNA 전사체를 조건화(conditioning)하는 방법.
- 제1항 내지 제4항 중의 어느 한 항에 있어서, 표적 서열을 포함하는 핵산을 프로모터 함유 분자와 하이브리드화하여 프로모터로부터의 전사 출발점에 대해 +6 이상에 상응하는 위치의 암호화 쇄에 닉을 형성시키는 방법.
- 제24항에 있어서, 닉이 +7, +8, +9 또는 +19의 위치에 존재하는 방법.
- 제1항에 있어서,a) 표적 핵산의 3'-말단에 있는 일본쇄 영역에 상보적인 암호화 쇄의 3'-말단에 5개 이상의 뉴클레오타이드를 포함하는 핵산 프로모터 함유 프로브를 고체 지지체상에 고정시키고;b) 서열화될 핵산을 고정된 핵산 프로브와 하이브리드화하고;c) 프로모터를 인지하는 RNA 폴리머라제를 사용하여 표적 핵산을 전사시켜 염기 특이적으로 종결된 다수의 RNA 전사체를 생성하며;d) 질량 분광분석법에 의해 염기 특이적으로 종결된 RNA 전사체 각각의 분자량을 측정함을 포함하는 방법.
- a) 표적 핵산의 3'-말단에 있는 일본쇄 영역에 상보적인 암호화 쇄의 3'-말단에 5개 이상의 뉴클레오타이드를 포함하는 핵산 프로모터 함유 프로브를 고체 지지체상에 고정시키고;b) 서열화될 핵산을 고정된 핵산 프로브와 하이브리드화하고;c) 프로모터를 인지하는 RNA 폴리머라제를 사용하여 표적 핵산을 전사시켜 서열 종결된 RNA 전사체를 생성하며;d) 질량 분광분석법에 의해 RNA 전사체의 분자량을 측정하여 터미네이터 서열 또는 어태뉴에이터를 확인함을 포함하여, 전사 터미네이터 서열 또는 어태뉴에이터 서열을 확인하는 방법.
Applications Claiming Priority (3)
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| US8/990,851 | 1997-12-15 | ||
| US08/990,851 | 1997-12-15 | ||
| US08/990,851 US6268131B1 (en) | 1997-12-15 | 1997-12-15 | Mass spectrometric methods for sequencing nucleic acids |
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| KR20010033130A true KR20010033130A (ko) | 2001-04-25 |
| KR100463459B1 KR100463459B1 (ko) | 2004-12-29 |
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| Country | Link |
|---|---|
| US (1) | US6268131B1 (ko) |
| EP (1) | EP1038031B1 (ko) |
| JP (1) | JP3331210B2 (ko) |
| KR (1) | KR100463459B1 (ko) |
| AT (1) | ATE255168T1 (ko) |
| AU (1) | AU745149B2 (ko) |
| CA (1) | CA2314906A1 (ko) |
| DE (1) | DE69820111T2 (ko) |
| NO (1) | NO20003058L (ko) |
| WO (1) | WO1999031278A1 (ko) |
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| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| KR20140134534A (ko) | 2013-05-14 | 2014-11-24 | 솔젠트 (주) | 유전자 검사에 기초하여 소아에게 권장 식이 정보를 제공하는 방법 및 이 방법에 사용되는 시스템 |
| KR20140136744A (ko) * | 2013-05-21 | 2014-12-01 | 솔젠트 (주) | 유전자 검사에 기초하여 신생아에게 권장 식이 정보를 제공하는 방법 및 이 방법에 사용되는 시스템 |
Also Published As
| Publication number | Publication date |
|---|---|
| AU745149B2 (en) | 2002-03-14 |
| US6268131B1 (en) | 2001-07-31 |
| EP1038031B1 (en) | 2003-11-26 |
| CA2314906A1 (en) | 1999-06-24 |
| WO1999031278A1 (en) | 1999-06-24 |
| KR100463459B1 (ko) | 2004-12-29 |
| ATE255168T1 (de) | 2003-12-15 |
| NO20003058L (no) | 2000-08-15 |
| DE69820111T2 (de) | 2004-08-19 |
| EP1038031A1 (en) | 2000-09-27 |
| NO20003058D0 (no) | 2000-06-14 |
| JP2002508192A (ja) | 2002-03-19 |
| DE69820111D1 (de) | 2004-01-08 |
| JP3331210B2 (ja) | 2002-10-07 |
| AU1918799A (en) | 1999-07-05 |
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